Variants of phosphotriesterase for the hydrolysis and detoxification of nerve agents

ABSTRACT

Variants of phosphotriesterase have been created that exhibit enhanced hydrolysis of V-type and G-type nerve agents over wild-type phosphotriesterase. V- and G-type nerve agents have an S P  and R P  enantiomer. The S P  enantiomers are more toxic. V-type nerve agents are among the most toxic substances known. Variants of phosphotriesterase can prefer to hydrolyze one enantiomer of VX over the other enantiomer.

GOVERNMENT LICENSE RIGHTS

This invention was made with government support under GM068550 awarded by National Institutes of Health and under HDTRA1-14-1-0004 awarded by the Defense Threat Reduction Agency. The government has certain rights in the invention.

FIELD

The disclosure relates generally to chemical warfare. More specifically, the disclosure relates to detoxification of organophosphate nerve agents.

BACKGROUND

The G-type (sarin, cyclosarin, and soman) and V-type (VX and VR) organophosphonates are among the most toxic compounds known. The toxicity of these compounds is due to their ability to inactivate acetylcholine esterase, an enzyme required for proper nerve function.(1) Acetylcholine esterase breaks down the neurotransmitter acetylcholine into acetic acid and choline. Acetylcholine conducts a nerve impulse between the nerve and the muscle, stimulating the muscle. The organophosphonate binds to the hydroxyl group on a serine at a binding site on acetylcholine esterase, preventing acetylcholine from binding at that site. If acetylcholine esterase is inhibited by an organophosphonate, acetylcholine builds up at the synapses and neuromuscular junctions and the receptor is desensitized resulting in paralysis with an estimated lethal dermal exposure of about 6 milligrams of VX for an average human.

Contact with VX is about 200-fold more toxic than soman (GD) and 300-fold more toxic than sarin (GB).(2) The extreme potential for acute toxicity with VX is due, in part, to the low volatility of this compound, which allows it to persist indefinitely on common surfaces.(3) Methods currently utilized for the destruction of organophosphate nerve agents include high temperature incineration and treatment with strong base or concentrated bleach.(4,5) Medical treatment of VX toxicity is currently limited to the injection of atropine, which reduces neurological symptoms, and oximes, which can help to reactivate the inactivated acetylcholine esterase.(2) Butyrylcholine esterase, which is closely related to acetylcholine esterase, has proven effective in animal models as a stoichiometric scavenger of VX.(6) However, the large amount of enzyme required for treatment with a stoichiometric scavenger, and the limited supply of this protein, have prevented butyrylcholine esterase from being an effective antidote for medical use.(7,8)

Enzymatic hydrolysis of nerve agents provides numerous advantages over harsh physical or chemical methods of decontamination and could provide a catalytic antidote for medical use. Enzymes such as organophosphorus acid anhydrolase (OPAA), diisopropyl-fluorophospatase (DFPase), and human paraoxonase (PON1) can hydrolytically neutralize the various G-type agents, (9,10,11,12) but except for PON1, they have no activity against the V-type agents.(11)

The enzyme phosphotriesterase (PTE) is capable of hydrolyzing a wide variety of organophosphonates including both the G-type and V-type nerve agents.(13,14) A substrate for PTE, the insecticide paraoxon (FIG. 3F) has an enzymatic efficiency that approaches the limits of diffusion (k_(cat)/K_(m)˜10⁸ M⁻¹ s⁻¹).(15)

The high toxicity and environmental persistence of VX makes the development of novel decontamination methods particularly important. PTE is capable of hydrolyzing VX. The enzymatic efficiency of PTE for VX is more than 5-orders of magnitude lower than with paraoxon. For the hydrolysis of the G-type agents by PTE, the values of k_(cat)/K_(m) are between 10⁴ and 10⁵ M⁻¹ s⁻¹.(13)

The G- and V-type nerve agents all contain a chiral phosphorus center where the S_(P)-enantiomers are significantly more toxic than the corresponding R_(P)-enantiomers.(16,17) In general, wild-type PTE preferentially hydrolyzes the R_(P)-enantiomers of these compounds. The overall selectivity depends on the relative size of the substituents attached to the phosphorus center, with larger differences in size resulting in greater stereoselectivity.(18)

Chiral chromophoric analogues of the G-type agents have been utilized to guide the evolution of PTE for the identification of variants that prefer the more toxic S_(P)-enantiomers of sarin, cyclosarin, and soman.(13,16,18) The catalytic activity of PTE for the more toxic S_(P)-enantiomer of cyclosarin (GF) has been increased by more than 4-orders of magnitude.(13) The catalytic efficiencies for the hydrolysis of the more toxic S_(P)-enantiomers by the enhanced variants of PTE for the hydrolysis of GB, GD, and GF approach 10⁶ M⁻¹ s⁻¹.(13)

Unfortunately, the activity of PTE against the V-type agents is about 3-orders of magnitude lower than that with the G-type agents (k_(cat)/K_(m)<10³ M⁻¹ s⁻¹). (14, 19). The net rate of VX hydrolysis by PTE is thought to be limited more by the chemistry of the leaving group than by the stereochemistry of the phosphorus center.(13,14,20) The X-ray crystal structure of PTE shows that this enzyme folds as a distorted (β/α)₈-barrel and that the bulk of the active site is formed from the 8 loops that connect the core β-strands to the subsequent α-helices.(21)

The twelve residues which make up the substrate binding site of PTE can be subdivided into three pockets that accommodate the small, large and leaving-group moieties of the substrate.(21)

The residues in the active site have been shown to be largely responsible for the observed substrate specificity.(22) Loop-7 is the largest of the loops that contribute to the substrate binding site, and is known to tolerate substantial sequence variation.(18,21,23) Previous attempts to evolve PTE for the hydrolysis of VX have utilized the insecticide demeton-S with modest success.(24,25)

It would be advantageous to have enzymes that could optimize the hydrolysis of organophosphate nerve agents, including a new analogue and mutation strategies to optimize PTE for the hydrolysis of G-agents and V-agents such as VX.

SUMMARY

An embodiment of the disclosure is a synthetic amino acid sequence comprising the synthetic amino acid sequence of VQFL (SEQ ID NO: 2), capable of hydrolyzing organophosphates. In an embodiment, a synthetic DNA sequence encodes the synthetic amino acid sequence of SEQ ID NO: 2. In another embodiment, a synthetic cDNA sequence comprises the coding sequence of the synthetic DNA. In another embodiment, a plasmid comprises the synthetic DNA sequence.

An embodiment of the disclosure is a method of hydrolysis of an organophosphate nerve agent comprising contacting an organophosphate nerve agent with the synthetic amino acid sequence SEQ ID NO: 2; and hydrolyzing the organophosphate nerve agent. In an embodiment, the organophosphate is VX. In another embodiment, the organophosphate is VR. In yet another embodiment, the organophosphate is selected from the group consisting of GB, GD, and GF.

An embodiment of the disclosure is a system for detoxifying an organophosphate nerve agent comprising contacting the synthetic amino acid sequence of SEQ ID NO: 2 with an organophosphate nerve agent.

An embodiment of the disclosure is a kit for detoxifying an organophosphate nerve agent comprising the synthetic amino acid sequence of SEQ ID NO: 2.

An embodiment of the disclosure is the synthetic amino acid sequence of claim 1, further comprising mutations I106C (CVQFL (SEQ ID NO: 3)). In an embodiment, a synthetic DNA sequence encodes the synthetic amino acid sequence of SEQ ID NO: 3. In an embodiment, a synthetic cDNA sequence comprises the coding sequence of the synthetic DNA sequence. In another embodiment, a plasmid comprises the synthetic DNA sequence.

An embodiment of the disclosure is a method of hydrolysis of an organophosphate nerve agent comprising contacting an organophosphate nerve agent with the synthetic amino acid sequence of SEQ ID NO: 3; and hydrolyzing the organophosphate nerve agent. In an embodiment, the organophosphate is VX. In another embodiment, the organophosphate is VR. In yet another embodiment, the organophosphate is selected from the group consisting of GB, GD, and GF.

An embodiment of the disclosure is a system for detoxifying an organophosphate nerve agent comprising contacting the synthetic amino acid sequence of SEQ ID NO: 3 with an organophosphate nerve agent.

An embodiment of the disclosure is a kit for detoxifying an organophosphate nerve agent comprising the synthetic amino acid sequence of SEQ ID NO: 3.

An embodiment of the disclosure is the synthetic amino acid sequence of claim 1, further comprising mutations A80V, K185R, and I274N (VRN-VQFL (SEQ ID NO: 4)). In an embodiment, the synthetic DNA sequence encodes the synthetic amino acid sequence of SEQ ID NO: 4. In another embodiment, the synthetic cDNA sequence comprises the coding sequence of the synthetic DNA sequence. In yet another embodiment, a plasmid comprises the synthetic DNA sequence.

An embodiment of the disclosure is a method of hydrolysis of an organophosphate nerve agent comprising contacting an organophosphate nerve agent with the synthetic amino acid sequence of SEQ ID NO: 4; and hydrolyzing the organophosphate nerve agent. In an embodiment, the organophosphate is VX. In an embodiment, the organophosphate is VR. In an embodiment, the organophosphate is selected from the group consisting of GB, GD, and GF.

An embodiment of the disclosure is a system for detoxifying an organophosphate nerve agent comprising contacting the synthetic amino acid sequence of SEQ ID NO: 4 with an organophosphate nerve agent.

An embodiment of the kit for detoxifying an organophosphate nerve agent comprising the synthetic amino acid sequence of SEQ ID NO: 4.

An embodiment of the disclosure is the synthetic amino acid sequence comprising the synthetic amino acid sequence of L7ep-3a (SEQ ID NO: 5). In an embodiment, a synthetic DNA sequence encodes the synthetic amino acid sequence of SEQ ID NO: 5. In an embodiment, a synthetic cDNA sequence comprises the coding sequence of the synthetic DNA sequence. In yet another embodiment, a plasmid comprises the synthetic DNA sequence.

An embodiment of the disclosure is a method of hydrolysis of an organophosphate nerve agent comprising contacting an organophosphate nerve agent with the synthetic amino acid sequence of SEQ ID NO: 5; and hydrolyzing the organophosphate nerve agent. In an embodiment, the organophosphate is VX. In an embodiment, the organophosphate is VR. In another embodiment, the organophosphate is selected from the group consisting of GB, GD, and GF.

An embodiment of the disclosure is a system for detoxifying an organophosphate nerve agent comprising contacting the synthetic amino acid sequence of SEQ ID NO: 5 with an organophosphate nerve agent.

An embodiment of the disclosure is a kit for detoxifying an organophosphate nerve agent comprising the synthetic amino acid sequence of SEQ ID NO: 5.

An embodiment of the disclosure is a synthetic amino acid sequence comprising the synthetic amino acid sequence of L7ep-3a I106G (SEQ ID NO.: 6), capable of hydrolyzing organophosphates. In an embodiment, a synthetic DNA sequence encodes the synthetic amino acid sequence of SEQ ID NO.: 6. In another embodiment, a synthetic cDNA sequence comprising the coding sequence of the synthetic DNA sequence. In yet another embodiment, a plasmid comprising the synthetic DNA sequence.

An embodiment of the disclosure is a method of hydrolysis of an organophosphate nerve agent comprising contacting an organophosphate nerve agent with the synthetic amino acid sequence of SEQ ID NO.: 6; and hydrolyzing the organophosphate nerve agent. In an embodiment, wherein the organophosphate is VX. In another embodiment, the organophosphate is VR. In yet another embodiment, the organophosphate is selected from the group consisting of GB, GD, and GF.

An embodiment of the disclosure is a system for detoxifying an organophosphate nerve agent comprising contacting the synthetic amino acid sequence of SEQ ID NO.: 6 with an organophosphate nerve agent.

An embodiment of the disclosure is a kit for detoxifying an organophosphate nerve agent comprising the synthetic amino acid sequence of SEQ ID NO.: 6.

An embodiment of the disclosure is a method of producing variants of phosphotriesterase, wherein the variants are capable of detoxifying an organophosphate nerve agent, comprising the steps of: obtaining a PTE gene; inserting the PTE gene into a vector; preparing a series of sequential mutational libraries wherein the PTE gene encodes a synthetic amino acid sequence of SEQ ID NO.: 6; expressing the variant as a protein; screening the variant for catalytic activity against one selected from the group consisting of DEVX, DMVX, DEVR, and OMVR to determine the hydrolytic activity; and selecting the variant for use in hydrolysis of an organophosphate nerve agent based upon its hydrolytic activity. In an embodiment, the variant synthetic amino acid sequence is at least 80% homogenous to the synthetic amino acid sequence of SEQ ID NO.: 6.

An embodiment of the disclosure is a method of producing variants of phosphotriesterase, wherein the variants are capable of detoxifying an organophosphate nerve agent, comprising the steps of: obtaining a PTE gene; inserting the PTE gene into a vector; preparing a series of sequential mutational libraries wherein the PTE gene encodes a synthetic amino acid sequence comprising the mutations I106C, F132V, H254Q, H257Y, A270V, L272M, I274N, and S308L (SEQ ID NO.: 5); expressing the variant as a protein; screening the variant for catalytic activity against one selected from the group consisting of DEVX, DMVX, DEVR, and OMVR to determine the hydrolytic activity; and selecting the variant for use in hydrolysis of an organophosphate nerve agent based upon its hydrolytic activity. In an embodiment, the variant comprising the mutations I106C, F132V, H254Q, H257Y, A270V, L272M, I274N, and S308L synthetic amino acid sequence is at least 80% homogenous to the synthetic amino acid sequence of SEQ ID NO.: 5)

The foregoing has outlined rather broadly the features of the present disclosure in order that the detailed description that follows can be better understood. Additional features and advantages of the disclosure will be described hereinafter, which form the subject of the claims.

BRIEF DESCRIPTION OF THE DRAWINGS

In order that the manner in which the above-recited and other enhancements and objects of the disclosure are obtained, a more particular description of the disclosure briefly described above will be rendered by reference to specific embodiments thereof which are illustrated in the appended drawings. Understanding that these drawings depict only typical embodiments of the disclosure and are therefore not to be considered limiting of its scope, the disclosure will be described with additional specificity and detail through the use of the accompanying drawings in which:

FIG. 1 depicts the hydrolysis of VX by phosphotriesterase to a nontoxic form;

FIG. 2A depicts the structure of (S_(P))-tabun (GA);

FIG. 2B depicts the structure of (S_(P))-sarin (GB);

FIG. 2C depicts the structure of (S_(P)S_(C))-soman (GD);

FIG. 2D depicts the structure of (S_(P)R_(C))-soman (GD);

FIG. 2E depicts the structure of paraoxon;

FIG. 2F depicts the structure of (S_(P))-cyclosarin (GF);

FIG. 2G depicts the structure of (S_(P))-VX;

FIG. 2H depicts the structure of (S_(P))-VR;

FIG. 3A depicts the structure of VX;

FIG. 3B depicts the structure of VR;

FIG. 3C depicts the structure of Demeton-S;

FIG. 3D depicts the structure of Demeton-S methyl;

FIG. 3E depicts the structure of diisopropyl amiton (DEVX);

FIG. 3F depicts the structure of paraoxon;

FIG. 3G depicts the structure of R_(P)-1;

FIG. 3H depicts the structure of S_(P)-1;

FIG. 4A depicts the structure of S_(P)-1 (Compound 1);

FIG. 4B depicts the structure of S_(P)-2 (Compound 2);

FIG. 4C depicts the structure of S_(P)-3 (Compound 3);

FIG. 4D depicts the structure of S_(P)S_(C)-4 (Compound 4);

FIG. 4E depicts the structure of S_(P)R_(C)-4 (Compound 4);

FIG. 4F depicts the structure of S_(P)-5 (Compound 5);

FIG. 4G depicts the structure of R_(P)-1 (Compound 1);

FIG. 4H depicts the structure of R_(P)-2 (Compound 2);

FIG. 4I depicts the structure of R_(P)-3 (Compound 3);

FIG. 4J depicts the structure of R_(P)R_(C)-4 (Compound 4);

FIG. 4K depicts the structure of R_(P)S_(C)-4 (Compound 4);

FIG. 4L depicts the structure of R_(P)-5 (Compound 5);

FIG. 5A depicts representative time courses for the complete hydrolysis of 160 μM racemic VX by the QF variant of PTE;

FIG. 5B depicts representative time courses for the complete hydrolysis of 160 μM racemic VX by the WT variant of PTE;

FIG. 5C depicts representative time courses for the complete hydrolysis of 160 μM racemic VX by the VRN-VQFL variant of PTE;

FIG. 5D depicts representative time courses for the complete hydrolysis of 160 μM racemic VX by the L7ep-3a variant of PTE;

FIG. 5E depicts representative time courses for the complete hydrolysis of 160 μM racemic VX by the L7ep-2b variant of PTE;

FIG. 5F depicts representative time courses for the complete hydrolysis of 160 μM racemic VX by the QF+L7ep-2b variant of PTE;

FIG. 6 depicts enhancement in the catalytic properties for the hydrolysis of VX and DEVX by variants of PTE;

FIG. 7 depicts representative Michaelis-Menton plots for the hydrolysis of DEVX by wild-type and evolved variants of PTE;

FIG. 8 depicts the hydrolysis of racemic VX by the VRN-VQFL variant observed by quantitative ³¹P{¹H} NMR spectroscopy;

FIG. 9 depicts construction of the multisite partially randomized PTE library;

FIG. 10 depicts the screening of the M317X mutant library against S_(P)-5 using GWT-d1 as the parental template.

FIG. 11A depicts screening of the six-site randomized library using GWT-f1 as the parental template with S_(P)-5;

FIG. 11B depicts screening of the error-prone PCR library using GWT-f4 as the parental template with S_(P)-5;

FIG. 12 depicts an outline of the parental linage for the construction of mutants of PTE that are enhanced for the hydrolysis of S_(P)-4 and S_(P)-5;

FIG. 13A depicts bar graphs illustrating enhanced values for k_(cat)/K_(m) (M⁻¹s⁻¹) for the S_(P)-enantiomer of compound 1 (FIG. 4A);

FIG. 13B depicts bar graphs illustrating enhanced values for k_(cat)/K_(m) (M⁻¹s⁻¹) for the S_(P)-enantiomer of compound 2 (FIG. 4B);

FIG. 13C depicts bar graphs illustrating enhanced values for k_(cat)/K_(m) (M⁻¹s⁻¹) for the S_(P)-enantiomer of compound 3 (FIG. 4C);

FIG. 13D depicts bar graphs illustrating enhanced values for k_(cat)/K_(m) (M⁻¹s⁻¹) for the S_(P)-enantiomer of compound S_(P)R_(C)-4 (compound 4) (FIG. 4E);

FIG. 13E depicts bar graphs illustrating enhanced values for k_(cat)/K_(m) (M⁻¹s⁻¹) for the S_(P)-enantiomer of compound S_(P)S_(C)-4 (compound 4) (FIG. 4D);

FIG. 13F depicts bar graphs illustrating enhanced values for k_(cat)/K_(m) (M⁻¹s⁻¹) for the S_(P)-enantiomer of compound 5 (FIG. 4F); and

FIG. 14 depicts the amino acid sequence of organophosphate-degrading protein (opd) from Brevundimonas diminuta (Pseudomonas diminuta) (SEQ ID NO: 1).

FIG. 15A depicts the structure of paraoxon.

FIG. 15B depicts the structure of S_(p)-APVR.

FIG. 15C depicts the structure of R_(p)-APVR.

FIG. 15D depicts the structure of S_(p)-VX.

FIG. 15E depicts the structure of DEVX.

FIG. 15F depicts the structure of DMVX.

FIG. 15G depicts the structure of S_(p)-VR.

FIG. 15H depicts the structure of DEVR.

FIG. 15I depicts the structure of R_(p)-OMVR.

FIG. 16A depicts a structural alignment between wild-type PTE (white) and L7ep-3a mutant (blue).

FIG. 16B depicts an expanded view of Loop-7 and -8.

FIG. 17 depicts the substrate binding pockets of wild-type (white) and L7ep-3a (grey).

FIG. 18 depicts the metal center of wild-type PTE (A), QF (B), and L7ep-3a (C) variants.

FIG. 19A depicts S_(P)-VX docked in thee active site of L7ep-3a.

FIG. 19B depicts S_(P)-VR docked into the active site of L7ep-3a I106G.

FIG. 20 depicts an equation of the interaction between S_(P)-VR and L7ep-3a PTE.

DETAILED DESCRIPTION

The particulars shown herein are by way of example and for purposes of illustrative discussion of the preferred embodiments of the present disclosure only and are presented in the cause of providing what is believed to be the most useful and readily understood description of the principles and conceptual aspects of various embodiments of the disclosure. In this regard, no attempt is made to show structural details of the disclosure in more detail than is necessary for the fundamental understanding of the disclosure, the description taken with the drawings making apparent to those skilled in the art how the several forms of the disclosure can be embodied in practice.

The following definitions and explanations are meant and intended to be controlling in any future construction unless clearly and unambiguously modified in the following examples or when application of the meaning renders any construction meaningless or essentially meaningless. In cases where the construction of the term would render it meaningless or essentially meaningless, the definition should be taken from Webster's Dictionary 3rd Edition.

As used herein the term, “wild-type” means and refers to the non-mutated version of a gene as it appears in nature.

As used herein the term, “enantiomer” means and refers to either of a pair of chemical compounds that have molecular structures that are nonsuperimposable mirror images.

As used herein the term, “G-agent” or “G-type” means and refers to nerve agents of the G (German) series. The series includes but is not limited to GA (tabun), GB (sarin), GF (cyclosarin) and GD (soman).

As used herein the term, “V-type” means and refers to nerve agents of the V series. The series includes but is not limited to VX, VE, V-gas, VG, VR, and VM.

Tables

Table 1. Mutations present in additional variants identified

Table 2. Activity of PTE Variants against VX Analogues DEVX and Compound 1 (R_(P)-1 and S_(P)-1) (see FIGS. 4A and 4G for structures)

Table 3. Activity of additional PTE Variants with DEVX

Table 4. Kinetic Parameters for PTE Variants with Paraoxon and Demeton-S

Table 5. Activity of PTE Variants with Racemic VX

Table 6. Identification of Mutants

Table 7. Activity of Wild-Type and Mutant Enzymes with Racemic G-Agents

Table 8. Kinetic Constants for Hydrolysis of GB, GD, and GF

Table 9. Values of k_(cat) (s⁻¹) for Wild-Type PTE and its Mutants

Table 10. Values of k_(cat)/K_(m) (M⁻¹ s⁻¹) for Wild-Type PTE and its Mutants

Table 11. Kinetic constants for PTE variants with APVR.

Table 12. Kinetic parameters for PTE variants with paraoxon and DEVX.

Table 13. Kinetic constants with the racemic nerve agents VX and VR.

Table 14. X-ray crystallography data for L7ep-3a and L7-ep-3a I106G.

Table 15. Kinetic constants for PTE variants with V-agent analogs.

The V-type organophosphorus nerve agents are among the most hazardous compounds known. Previous efforts to evolve the bacterial enzyme phosphotriesterase (PTE) for the hydrolytic decontamination of VX resulted in the variant L7ep-3a, which has a k_(cat) value more than 2-orders of magnitude higher than wild-type PTE. Because of the relatively small size of the O-ethyl, methylphosphonate center in VX, stereoselectivity is not a major concern. However, the Russian V-agent, VR, contains a larger 0-isobutyl, methylphosphonate center making stereoselectivity a significant issue since the S_(P)-enantiomer is more toxic than the R_(P)-enantiomer. The three-dimensional structure of the L7ep-3a variant was determined to a resolution of 2.01 Å (PDB id: 4ZST). The active site of the L7ep-3a mutant has revealed a network of hydrogen bonding interactions between Asp-301, Tyr-257, Gln-254 and the hydroxide that bridges the two metal ions. A series of new analogs that mimic VX and VR has helped to identify critical structural features for the development of new enzyme variants that are further optimized for the catalytic detoxification of VR and VX. The best of these mutants has been shown to hydrolyze the more toxic S_(P)-enantiomer of VR more than 600-fold faster than the wild-type phosphotriesterase. The organophosphorus nerve agents are among the most toxic compounds known. Compounds such as sarin, soman and VX are all chiral methyl phosphonates where the toxicity of the SP-enantiomer is much greater than for the RP-enantiomer.(33) Recent events have dramatically demonstrated the continuing importance of developing rapid and environmentally compatible methods for the decontamination of these compounds.(34) This situation is particularly true for the V-type nerve agents, where the lethal dose is approximately 6 mg/person, and these compounds have been shown to persist for long periods of time.(35, 36) Significant advances have been made in developing enzymatic methods of decontamination for the G-type and VX nerve agents using the bacterial enzyme phosphotriesterase (PTE).(37, 38) While wild-type PTE has reasonable activity against the G-type nerve agents (kcat/Km˜105 M−1 s−1), this enzyme preferentially hydrolyzes the less toxic R_(P)-enantiomers.(39) Directed evolution of PTE to specifically target the G-type nerve agents has led to the identification of the variant H257Y/L303T (YT), which has proven highly efficient at the hydrolysis of the more toxic S_(P)-enantiomer of sarin (GB), soman (GD), and cyclosarin (GF) with values of k_(cat)/K_(m) that exceed 106 M⁻¹ s⁻¹.(38)

Wild-type PTE exhibits little stereoselectivity against the relatively small phosphonate center of VX, but the elevated pK_(a) of the thiol-leaving group provides a significant challenge for enzyme-catalyzed hydrolysis (k_(cat)/K_(m)˜102 M⁻¹ s⁻¹).(37) Mutation of residues contained within the active site of PTE resulted in the isolation of the variant H245Q/H257F (QF), which exhibited a 100-fold improvement for the hydrolysis of VX, relative to the wild-type enzyme (see Table 1 for identity of variants).(37) Additional active site variations resulted in the identification of the mutant CVQFL (QF+I106C/F132V/S308L) with a similar catalytic efficiency for the hydrolysis of VX, but a three-fold improvement in k_(cat). The best variant identified to date for the hydrolysis of VX is VRN-VQFL (QF+F132V/S308L+A80V/K185R/1274N). This mutant combines expression-enhancing mutations (A80V/K185R/1274N) with additional changes in the active site to achieve a k_(cat)/K_(m) of 7×10⁴ M⁻¹ s⁻¹ for the hydrolysis of the S_(P)-enantiomer of VX. (37, 40, 41) Expansion of the mutation strategy to targeted error-prone PCR, led to the identification of the variant L7ep3a (CVQFL+H257Y/A270V/L272M/I274N), which has a k_(cat) value enhanced 152-fold relative to wild-type PTE.(37) How these combined mutations, some of which do not fall in the active site, are able to bring about such a dramatic improvement in catalytic ability is not clear.

In addition to VX, the V-agents include the Russian (VR) and Chinese versions. Exemplified by VR, these additional V-agents contain a smaller thiol leaving group, and a larger ester group attached to the phosphorus center (FIGS. 15A-15I). Wild-type PTE has enzymatic activity for the hydrolysis of racemic VR similar to VX, but the larger isobutyl group attached to the phosphorus center results in a 25-fold preference for the less toxic R_(P)-enantiomer.(39, 42) The catalytic activity of wild-type PTE for the hydrolysis of the more toxic S_(P)-enantiomer of VR (k_(cat)/K_(m)=4.3 M−1 s−1) is significantly lower than for the hydrolysis of VX. PTE variants which contain many of the same mutations as the VX-enhanced variants have been reported to have substantially improved catalytic activity against S_(P)-VR.(43) Currently, there is a lack of three-dimensional structural data that can be used to explain how the existing set of mutants are able to enhance the rate of hydrolysis of the phosphorothiolate bond in VX.

PTE variants can be used to decontaminate areas, equipment, and personnel after they come in contact with V-type or G-type nerve agents. This is especially useful for military or homeland security applications. The decontamination occurs without exposing the area, equipment, or personnel to harsh chemicals. Mutations in the sequence of PTE have been made to increase the ability of PTE to hydrolyze, and thus decontaminate, an area, equipment, or personnel. PTE was subjected to directed evolution for the improvement of catalytic activity against selected compounds through the manipulation of active site residues. A series of sequential two-site mutational libraries encompassing twelve active site residues of PTE was created. The libraries were screened for catalytic activity against a new VX analogue (DEVX), which contains the same thiolate leaving group of VX coupled to a di-ethoxy phosphate core rather than the ethoxy, methylphosphonate core of VX. The catalytic activity with DEVX was enhanced 26-fold relative to wild-type PTE. Further improvements were facilitated by targeted error-prone PCR mutagenesis of Loop-7 and additional PTE variants were identified with up to a 78-fold increase in the rate of DEVX hydrolysis. The best mutant hydrolyzed the racemic nerve agent VX with a value of k_(cat)/K_(m) of 7×10⁴ M⁻¹ s⁻¹; a 230-fold improvement relative to the wild-type PTE. The sequence of wild-type PTE (organophosphate-degrading protein (opd)), without the leader peptide residues (1-29), is found in FIG. 14. The highest turnover number achieved by the mutants tested was 137 s⁻¹; an enhancement of 152-fold relative to wild-type PTE. The stereoselectivity for the hydrolysis of the two enantiomers of VX was relatively low.

The P—S bond in VX is chemically more stable than the P—F bond found in the G-agents.(20) (FIGS. 2G, 2A-2D) Demeton-S contains the requisite P—S bond but does not contain the tertiary amine of VX, which is likely to be protonated at the relevant pH values. (FIGS. 3C, 3A) DEVX, containing the authentic leaving group of VX, yields results more directly applicable to the hydrolysis of VX itself. (FIGS. 3E, 3A)

The QF variant of PTE shows improved hydrolysis against the SP-enantiomer of a chiral VX analogue.(18) Table 1 lists the amino acid changes present in the variants. This mutant was found to be significantly better for the hydrolysis of the P—S bond in DEVX and demeton-S than wild-type PTE. The synergistic mutations in this variant suggested that further improvements in catalytic activity could be facilitated by simultaneously mutating pairs of residues in the active site. The initial mutant libraries targeted pairs of residues in the active site that modulated the size and shape of the three substrate binding pockets. Sequential optimization of the active site residues resulted in an 18-fold improvement in catalytic activity against DEVX. Combining the best variant (VQFL) with expression enhancing mutations resulted in the variant VRN-VQFL. The VRN-VQFL variant exhibited a 26-fold improvement for the hydrolysis of DEVX.

TABLE 1 Mutations present in additional variants identified. Variant Mutations present WT Wild type ARN A80V/K185R/I274N QF H254Q/H257F QF.1 H254Q/H257F/F306W/Y309H LQF F132L/H254Q/H257F VQF F132V/H254Q/H257F QF.a W131H/F132L/H254Q/H257F QF.b W131H/F132I/H254Q/H257F LQF.1 F132L/H254Q/H257L LQF.2 F132L/H254R/H257A LQF.3 F132L/H254R/H257L LQF.4 F132L/H254R/H257Y LQF.a F132L/H254Q/H257F/L271V LQF.b F132L/H254Q/H257F/L271M LQF.c F132L/H254Q/H257F/L271A LQFL F132L/H254Q/H257F/S308L LQF.d F132L/H254Q/H257F/L271R/S308N VQFL F132V/H254Q/H257F/S308L CVQFL I106C/F132V/H254Q/H257F/S308L VQFL.1 I106G/F132V/H254Q/H257F/S308L VQFL.2 I106S/F132V/H254Q/H257F/S308L VQFL.3 I106A/F132V/H254Q/H257F/L303T/S308L VRN-VQFL A80V/F132V/K185R/H254Q/H257F/I274N/S308L VRNGS-VQFL A80V/F132V/K185R/D208G/H254Q/H257F/I274N/ S308L/R319S L7ep-1 F132V/H254S/H257W/A266T/L271P/S308L L7ep-2 I106C/F132V/H254R/H257F/N265D/A270D/L272M/ S276T/S308L L7ep-3 I106C/F132V/H254Q/H257Y/A270V/L272M/S308L L7ep-4 I106C/F132V/H254Q/H257F/I260N/D264N/I274N/ S308L L7ep-5 I106C/F132V/H254Q/H257Y/E264G/S308L L7ep-6 I106C/F132V/H254Q/H257F/A266E/S269T/S308L L7ep-7 I106C/F132V/H254Q/H257F/I260V/S269T/S308L L7ep-8 I106C/F132V/H254Q/H257Y/I260V/S308L L7ep-9 I106C/F132V/H254Q/H257F/S269T/I274T/S308L L7ep-10 I106C/F132V/H254Q/H257Y/E263K/S308L L7ep-11 I106C/F132V/H254Q/H257Y/A266R/S308L L7ep-12 I106C/F132V/H254Q/H257F/S269T/I274S/S308L L7ep-2a I106C/F132V/H254R/H257F/N265D/A270D/L272M/ I274T/S276T/S308L L7ep-2b I106C/F132V/H254R/H257F/N265D/A270D/I274N/ S276T/S308L L7ep-2c I106C/F132V/H254Q/H257F/N265D/A270D/L272M/ S276T/S308L L7ep-2d I106C/F132V/H254R/H257F/N265D/A270D/L272M/ I274S/S276T/S308L L7ep-2e I106C/F132V/H254R/H257F/N265D/A270D/I274P/ S276T/S308L L7ep-2f I106C/F132V/H254R/H257F/N265D/A270D/I274S/ S276T/S308L L7ep-2g I106C/F132V/H254R/H257F/N265D/A270D/I274Q/ S276T/S308L L7ep-2h I106C/F132V/H254R/H257F/N265D/A270D/L272M/ S276H/S308L L7ep-2i I106C/F132V/H254R/H257F/N265D/A270D/L272M/ S276S/S308L L7ep-2j I106C/F132V/H254R/H257F/N265D/A270D/L272M/ S276P/S308L L7ep-3a I106C/F132V/H254Q/H257Y/A270V/L272M/I274N/ S308L L7ep-3b I106C/F132V/H254Q/H257Y/A270D/L272M/S308L L7ep-3c I106C/F132V/H254Q/H257Y/N265D/L272M/S308L L7ep-3d I106C/F132V/H254Q/H257Y/A270V/L272M/I274T/ S308L

Additional strategies were used to further enhance the activity of PTE against the phosphorothiolate bond. Error-prone PCR is a useful technique for enzyme evolution, but the mutation frequencies are typically restricted to 1-3 base pair changes per gene because of the significant chance of introducing deleterious mutations. Substantial improvements in enzyme activity can require numerous amino acid changes, which are not typically achievable by error-prone PCR. Targeting error-prone PCR to only Loop-7 (residues 253-276) resulted in a mutation library with an average of 6 mutations per gene but still retained>20% active colonies. The hydrolysis of DEVX for one of the variants (L7ep-3) was improved to 36-fold over wild-type PTE due to 3 additional amino acid changes. The best variant identified (L7ep-2) was improved 63-fold for the hydrolysis of DEVX by 5 additional amino acid changes. Further optimization of L7ep-2 and L7ep-3 resulted in additional mutations that improved the activity to 78-fold (L7ep-2a) and 71-fold (L7ep-3a) over wild-type PTE, and achieved turnover numbers for the hydrolysis of the phosphorothiolate bond in excess of 100 s⁻¹.

Hydrolysis of VX. A full kinetic characterization of wild-type and improved variants of PTE using racemic VX was conducted. Wild-type PTE exhibited low activity against VX, but there was a dramatic improvement with the QF mutant. The mutations in the large group pocket resulted in substantial improvements to k_(cat). The best variant identified (VRN-VQFL) against VX combines active site mutations in all three pockets and has a k_(cat)/K_(m) value that is increased 235-fold over wild-type PTE (FIG. 6). FIG. 6 depicts enhancement in the catalytic properties for the hydrolysis of VX and DEVX by variants of PTE. The values of k_(cat)/K_(m) for evolved variants of PTE are presented for DEVX (open bars) and VX (cross-hatched bars). The k_(cat) values for the hydrolysis of VX are shown as right-hatched bars. (FIG. 6).

The Loop-7 optimized variants show good activity against VX, but did not demonstrate improved activity relative to the VRN-VQFL variant. The changes to Loop-7 resulted in substantial improvements in k_(cat) but little change in the catalytic efficiency.

The L7ep-3a variant has a k_(cat) of 137 s⁻¹ for the hydrolysis of VX. This value is the highest ever reported for the enzymatic hydrolysis of VX.(11,14,24,25) Single concentration experiments with the H254R/H257L mutant of PTE showed an improvement of 10-fold against racemic VX.(24) Another variant exhibited a 26-fold improvement over wild-type PTE at 0.5 mM VX.(25) By contrast, the VRN-VQFL and L7ep-3 variants are improved by more than 200-fold in the value of k_(cat)/K_(m). Human PON1 (paraoxonase) has been evolved in the laboratory for the hydrolysis of VX, but the reported value of k_(cat)/K_(m) for the best variant is 2.5×10³ M⁻¹ s⁻¹, whereas the best PTE variant (VRN-VQFL) identified in this investigation has a value of k_(cat)/K_(m) of 7×10⁴ M⁻¹ s⁻¹.(11)

Stereochemical Preferences of Active Site Mutants. The toxicity of the organophosphate nerve agents depends on the stereochemistry of the phosphorus center.(17) With VX, it is estimated that the S_(P)-enantiomer is about 100-fold more toxic than the R_(P)-enantiomer. The QF mutant prefers to hydrolyze the more toxic S_(P)-enantiomer of VX by a factor of 12, relative to the R_(P)-enantiomer, whereas the L7ep-2b mutant prefers to hydrolyze the R_(P)-enantiomer by a factor of 12. The stereochemical preferences for the hydrolysis of VX are fully consistent with the stereoselective properties of these two mutants for the hydrolysis of S_(P)-1 and R_(P)-1, suggesting that the variants VRN-VQFL, L7ep-3, and L7ep-3a also prefer the S_(P)-enantiomer of VX. While the modest selectivity prevented definitive assignment of the preferred enantiomer, complete neutralization of VX by the VRN-VQFL mutant via the hydrolysis of both enantiomers was demonstrated by 31^(P)-NMR spectroscopy (FIG. 8).

The reconstruction of PTE for the hydrolysis of VX has resulted in dramatic improvements in the values of k_(cat) and k_(cat)/K_(m), relative to the wild type enzyme. It is proposed that the increase in the catalytic constants has been achieved by an increase in the rate constant for cleavage of the P—S bond (k₃) rather than changes in the formation of the ternary complex (k₁, k₂) or the rate constant for product release (k₅) as illustrated in a minimal kinetic mechanism (Scheme 1). The thiol leaving group of VX has a higher pK_(a) than the fluoride leaving group of the G-agents, and the p-nitrophenol group of paraoxon. It has been demonstrated with the wild-type PTE that the chemical step (k₃) is rate limiting for substrates with leaving groups having pK_(a) values higher than 8.(20) Disruption of the hydrogen bonded network from D301-H254-D233 reduced the rate of hydrolysis of substrates with leaving groups having low pK_(a) values but increased the rate of hydrolysis of substrates with leaving groups of higher pK_(a) values.(30) Introduction of a glutamine at residue position 254 (as in the initial QF mutant), which apparently cannot support the transport of a proton away from the active site, may now facilitate the protonation of the thiol group by Asp-301 as the phosphorothiolate bond is cleaved.

The turnover numbers for some slow substrates of PTE are thought to be reflective of the ability of the enzyme to align the substrate with the nucleophilic hydroxyl group attached to the binuclear metal center.(13) There is a strong likelihood that for some of the variants, subtle changes in the conformation of the active site will facilitate a better alignment between the substrate and attacking hydroxide, thereby achieving higher enzymatic rates of hydrolysis. In particular, the Loop-7 variants have been modified at residues that are somewhat distant from the active site, but are expected to bring about changes in the positioning of the Loop-7 α-helix.(13,28) This alignment effect would, of course, differ between the di-ethoxy phosphorus center of DEVX and the methylphosphonate core of VX (FIGS. 3E, 3A), which may explain the differences in the k_(cat) values for DEVX and VX with the variants L7ep-2a and L7ep-3a. (Table 2) These changes have resulted in variants with high enzymatic efficiency and exceptional kinetic constant for the hydrolysis of VX.

TABLE 2 Activity of PTE Variants against VX analogues DEVX and compound 1 (see FIGS. 3, 4A and 4G for structures)* DEVX R_(P)-1 S_(P)-1 Variant k_(cat) K_(m) k_(cat)/K_(m) k_(cat) K_(m) k_(cat)/K_(m) k_(cat) K_(m) k_(cat)/K_(m) WT 1.1 0.87 1.2 × 10³ 100 3700 2.7 × 10⁴ 92 320 2.9 × 10⁵ QF 6.1 1.4 4.2 × 10³ 120 230 5.3 × 10⁵ 34 18 1.8 × 10⁶ LQF 15 1.7 9.0 × 10³ 112 910 1.2 × 10⁵ 27 13 2.1 × 10⁶ VQF 18 1.0 1.9 × 10⁴ 82 340 2.4 × 10⁵ 25 11 2.2 × 10⁶ LQFL 10 0.76 1.4 × 10⁴ 76 160 4.7 × 10⁵ 45 7.4 6.1 × 10⁶ VQFL 14 0.65 2.2 × 10⁴ 69 129 5.3 × 10⁵ 32 7.4 4.3 × 10⁶ CVQFL 16 0.76 2.1 × 10⁴ 54 170 3.2 × 10⁵ 39 24 1.6 × 10⁶ VRN-VQFL 22 0.73 3.1 × 10⁴ 124 160 7.8 × 10⁵ 65 26 2.5 × 10⁶ VRNGS-VQFL 11 0.99 1.1 × 10⁴ 204 350 5.8 × 10⁵ 93 22 4.3 × 10⁶ L7ep-1 16 0.60 3.2 × 10⁴ 590 8600 6.8 × 10⁵ 670 2800 2.3 × 10⁵ L7ep-2 48 0.63 7.6 × 10⁴ 240 730 3.3 × 10⁵ 90 400 2.3 × 10⁵ L7ep-3 29 0.69 4.3 × 10⁴ 143 560 2.5 × 10⁵ 50 22 2.3 × 10⁶ L7ep-2a 135 1.4 9.4 × 10⁴ 235 950 2.5 × 10⁵ 180 1090 1.7 × 10⁵ L7ep-2b 76 1.0 7.4 × 10⁴ 136 610 2.2 × 10⁵ 95 1090 8.6 × 10⁴ L7ep-3a 51 0.6 8.5 × 10⁴ 290 1500 1.9 × 10⁵ 90 36 2.5 × 10⁶ L7ep-36 64 1.0 6.2 × 10⁴ 202 1800 1.1 × 10⁵ 48 34 1.4 × 10⁶ *Standard errors from fits of the data to eq 1 are less than 20% of the stated values.

The structure of the L7ep3a variant was determined. The structure aided in understanding the chemical mechanism for the enhancement of phosphorothiolate bond cleavage. With this new structural information, a series of PTE variants was created to incorporate changes in the active site of PTE that would more easily accommodate the O-isobutyl group of VR. To facilitate the further development of PTE for the hydrolysis of various V-agents, a new series of analogs were designed and synthesized. Enhanced variants of PTE have been identified that have more than a 600-fold improvement in the catalytic activity for the hydrolysis of the toxic SP-enantiomer of VR.

EXAMPLES Example 1

Most chemicals can be obtained from Sigma Chemical Company. The pfuTurbo DNA polymerase can be obtained from Agilent Technologies and the various restriction enzymes can be acquired from New England Biolabs. The two enantiomers of compound 1 (FIGS. 4A and 4G) can be synthesized.(18) VX samples can be Chemical Agent Standard Analytical Reference Material (CASARM).

Example 2

Active Site Library Construction. The nucleotides in the gene for PTE were modified to replace the nucleotides encoding the leader peptide (amino acid residues 1-29) with nucleotides encoding a methionine. (FIG. 14) Nucleotides encoding amino acid residues 29-365 of PTE were inserted into a pET 20b+ vector between the NdeI and EcoRI restriction sites as previously described.(18) The amino acid residue numbering of the sequence including the leader sequence has been retained. The 306X/309X, 131X/132X and 254X/257X double substitution libraries were constructed by site-directed mutagenesis using single sets of primers containing NNS (N=any base, S=G or C) codons at the positions of interest. The 271X/308X library was constructed by sequential reactions. The 106X/303X and 60X/317X libraries were constructed using a PCR overlap extension technique.(26) Plasmids from at least 10 colonies of each library were sequenced to ensure the randomization at the positions of interest. The identities of specific mutations for the variants are given in Table 1. The name of the phosphotriesterase gene is opd, the GenBank Accession Number is AER10490.1, and the Protein Model Portal Accession Number is G8DNV8.

Example 3

Construction of Targeted Error-Prone Library. To construct the Loop-7 error-prone library, a set of 30-bp primers corresponding to the DNA sequences upstream and downstream of Loop-7 (amino acid residues 253-276) were used to amplify the PTE gene in three fragments. The amino acid residue numbering of the sequence including the leader sequence has been retained. The DNA coding region of Loop-7 was amplified in an error-prone PCR reaction while the two remaining fragments were amplified using standard PCR techniques. The final gene was constructed using PCR overlap-extension, resulting in a gene library with errors only in the coding region for residues 253-276.

Example 4

Optimization of Error-Prone Variants. The five residue positions (254, 265, 270, 272, and 276) identified in the best Loop-7 error prone variant and residues 257 and 274 were further optimized by construction of two two-site (254X/257X and 272X/274X) and three single-site libraries (265X, 270X, 276X). The amino acid residue numbering of the sequence including the leader sequence has been retained. Libraries were constructed via QuikChange mutagenesis using degenerate primers to allow all 20 amino acids at the positions of interest. Approximately 200 colonies from each single-site library were screened, and approximately 1200 colonies from each two-site library were screened. The two enhanced variants identified in the Loop-7 error prone library were used as the template for a second round of targeted error-prone PCR of Loop-7.

Example 5

Library Screening. Plasmid libraries were transformed into BL21 (DE3) E. coli competent cells and grown on LB plates. For all library transformations, the amount of DNA was kept low (<10 ng) to avoid the potential complication of double transformants.(27) Single colonies were used to inoculate 0.75 mL cultures of Super Broth (32 g tryptone, 20 g yeast extract, 5 g NaCl, and 0.4 g NaOH in 1 L H₂O) supplemented with 0.5 mM CoCl₂ in a 96-well block format. Cultures were grown at 37° C. for 8 hours. The temperature was reduced to 30° C. and protein expression induced by addition of 1 mM IPTG. Following 16 hours of additional growth, the bacteria were harvested by diluting a portion of the culture in a 1:1 ratio with 50 mM HEPES pH 8.0, 100 μM CoCl₂, 10% BugBuster® 10× (EMD Chemicals). Cultures were tested for activity against DEVX using a standard 250 μL assay that consisted of 50 mM HEPES, pH 8.0, 100 μM CoCl₂, 0.3 mM 5,5′-dithiobis(2-nitro-benzoic acid)(DTNB) and 0.2-0.5 mM DEVX. The reactions were initiated by the addition of 10 μL of cell lysate. Reactions proceeded at room temperature until color was clearly visible (1-4 hours). Product formation was determined by the change in absorbance at 412 nm using a plate reader. The variant used as the starting template for each library was included as a control on each plate. To account for differential culture growth, the final change in absorbance was normalized using the OD₆₀₀ for each culture compared to the average OD₆₀₀ of controls. The colonies giving the best results were re-grown as 5 mL overnight cultures and the plasmids harvested and sequenced to identify the variants.

Example 6

Kinetic Measurements. All assays with DEVX, paraoxon, S_(P)-1, R_(P)-1, and demeton-S were 250 μL in total volume and followed for 15 minutes in a 96-well plate reader at 30° C. Assays with VX were conducted in a volume of 500 μL in 1 mL cuvettes. DEVX, demeton-S, and VX assays monitored the release of the product thiol at 412 nm (Δε₄₁₂=14,150 M⁻¹ cm⁻¹) by the inclusion of DTNB in the reaction mixture (50 mM HEPES, pH 8.0, 100 μM CoCl₂, and 0.3 mM DTNB). Assays with paraoxon and compound 1 (FIGS. 4A and 4G) were conducted in 50 mM CHES, pH 9.0, and 100 μM CoCl₂. Assays of compound 1 (FIGS. 4A and 4G) contained 10% methanol. Paraoxon hydrolysis was followed by the release of p-nitrophenol at 400 nm (Δε₄₀₀=17,000 M⁻¹ s⁻¹) and the hydrolysis of compound 1 (FIGS. 4A and 4G) was followed at 294 nm (Δε₂₉₄=7,710 M⁻¹ cm⁻¹). Reactions were initiated by the addition of enzyme. The data were fit to equation 1 to obtain values of K_(m), k_(cat), and k_(cat)/K_(m). A representative data set is provided in FIG. 7. FIG. 7 depicts representative Michaelis-Menton plots for the hydrolysis of DEVX by wild-type and evolved variants of PTE. Reaction conditions were 50 mM Hepes (pH 8), 100 μM CoCl₂, 0.3 mM DTNB in a total volume of 250 μL at 30° C. (FIG. 7). Reactions were initiated by addition of appropriately diluted enzyme. Enzyme concentrations in the reactions were; wild-type=54 nM, CVQFL=5.0 nM, VRN-VQFL=6.29 nM, L7ep-3a=1.88 nM, and L7ep-2a 2.26 nM. The solid line represents the fit of the data to equation 1.

v/E _(t) =k _(cat)(A)/(K _(m) +A)  (Equation 1)

Example 7

Stereoselective Hydrolysis of Racemic VX. Low initial concentrations (19 to 160 μM) of racemic VX were hydrolyzed by variants of PTE in a solution containing 0.1 mM CoCl₂, 0.3 mM DTNB, and 50 mM Hepes, pH 8.0. The reactions were followed to completion and the fraction of VX hydrolyzed plotted as a function of time. The time courses were fit to equations 2 and 3 where F is the fraction of substrate hydrolyzed, a and b are the magnitudes of the exponential phases, t is time, and k₁ and k₂ are the rate constants for each phase.

F=a(1−e ^(−k) ¹ ^(t))  (Equation 2)

F=a(1−e ^(−k) ¹ ^(t))+b(1−e ^(−k) ² ^(t))  (Equation 3)

To identify which one of the two enantiomers of VX was preferentially hydrolyzed by the PTE variants, one gram of racemic VX was hydrolyzed in a 400 mL reaction mixture containing 50 mM bis-tris-propane (pH 8.0), 100 μM CoCl₂, and 36 nM of the QF mutant (H254Q/H257F) at 33° C. The reaction was monitored by determining the concentration of the thiol product with DTNB. When the reaction was approximately 50% complete, the remaining VX was extracted with 200 mL of ethyl acetate. The volume of the extract was reduced to approximately 2 mL by rotary evaporation at 41° C. The unreacted VX was analyzed with a polarimeter and observed to rotate plane polarized light in a positive direction (+0.055° to +0.075°) which corresponds to an enantiomeric preference for hydrolysis of the S_(P)-enantiomer of VX by the QF mutant.(17)

Example 8

Construction and Screening of Active Site Libraries. The variant QF (H254Q/H257F) was previously identified as being improved against the chiral centers in VX and VR.(18) Testing the catalytic activity of this mutant with the VX analogue, DEVX, revealed that this variant has an enhanced activity for the hydrolysis of the phosphorothiolate bond, relative to wild-type PTE. The amino acid residue numbering of the sequence including the leader sequence has been retained. The variant QF then served as the starting point for the construction of the F306X/Y309X and W131X/F132X double-substitution protein libraries. Screening 920 colonies from the F306X/Y309X library with DEVX failed to identify any variant that was improved relative to the QF parent. From the W131X/F132X library, a total of 1100 colonies were screened with DEVX and the two best mutants were identified as LQF (QF+F132L) and VQF (QF+F132V). The LQF variant served as the starting template for the 254X/257X library. Approximately 1650 colonies were screened from this library with DEVX, but none proved to be better for the hydrolysis of DEVX.

The 271X/308X library was created using sequential QuikChange procedures; first at position 271 then at position 308 using the LQF template. Approximately 2200 colonies from this library were screened and the best variant was LQFL (LQF+S308L). Incorporation of the new mutation (S308L) into the previously identified VQF variant further enhanced the catalytic activity. The variant VQFL (VQF+S308L) was utilized as the parent for the 106X/303X library. Approximately 1100 colonies were screened with DEVX and the best variant identified was CVQFL (VQFL+I106C). The variant CVQFL was carried forward in the construction of the 60X/317X library. Nearly 1500 colonies from this library were screened with DEVX, but improved variants were not detected.

A number of mutations are known to improve protein expression levels for PTE, including A80V, K185R, and I274N.(28,29) These mutations do not typically result in significant changes in the kinetic constants for a given substrate, but they dramatically improve the amount of enzyme produced per liter of cell culture. Adding these expression-enhancing mutations to VQFL resulted in an additional variant, VRN-VQFL (A80V/K185R/I274N+VQFL) with a 26-fold improvement in the value of k_(cat)/K_(m), relative to the wild-type PTE. The inclusion of two additional expression-enhancing mutations (D208G/R319S) resulted in a decrease in catalytic activity.(29) Kinetic constants for the PTE variants with DEVX as the target substrate are presented in Table 2. Kinetic constants for additional variants are provided in Table 3.

TABLE 3 Activity of additional PTE Variants with DEVX. Variant k_(cat)(s⁻¹) K_(m)(mM) k_(cat)/K_(m)(M⁻¹s⁻¹) QF.1 0.67 ± 0.01  2.2 ± 0.1 (3.05 ± 0.01) × 10² QF.a 1.23 ± 0.02  2.3 ± 0.1 (5.35 ± 0.02) × 10² QF.b  0.7 ± 0.2  1.9 ± 0.1 (3.9 ± 0.1) × 10³ LQF.1 10.1 ± 0.2 2.32 ± 0.08 (4.4 ± 0.2) × 10³ LQF.2  4.2 ± 0.2  4.1 ± 0.3 (1.02 ± 0.08) × 10³ LQF.3  8.4 ± 0.3  3.0 ± 0.2 (2.8 ± 0.2) × 10³ LQF.4 21.7 ± 0.4 2.91 ± 0.09 (7.5 ± 0.2) × 10³ LQF.a  9.4 ± 0.2 1.62 ± 0.07 (5.8 ± 0.3) × 10³ LQF.b 14.5 ± 0.4  2.8 ± 0.1 (5.2 ± 0.3) × 10³ LQF.c 25.2 ± 0.8  2.8 ± 0.2 (9.2 ± 0.6) × 10³ LQF.d  4.1 ± 0.3   13 ± 1 (3.1 ± 0.4) 10×² VQFL.1 24.9 ± 0.5  2.0 ± 0.1 (1.23 ± 0.05) × 10⁴ VQFL.2 20.4 ± 0.6  2.6 ± 0.1 (7.9 ± 0.5) × 10³ VQFL.3 0.93 ± 0.03  2.3 ± 0.1 (4.1 ± 0.3) × 10² L7ep-4 18.8 ± 0.3 0.89 ± 0.03 (2.11 ± 0.08) × 10⁴ L7er-5 13.4 ± 0.1 1.06 ± 0.02 (1.26 ± 0.03) × 10⁴ L7ep-6 17.2 ± 0.2 0.63 ± 0.02 (2.73 ± 0.08) × 10⁴ L7ep-7 18.4 ± 0.2 0.66 ± 0.02 (2.81 ± 0.09) × 10⁴ L7ep-8 16.2 ± 0.3 1.11 ± 0.04 (1.45 ± 0.05) × 10⁴ L7ep-9 16.3 ± 0.2 0.54 ± 0.02 (3.0 ± 0.1) × 10⁴ L7ep-10  9.6 ± 0.1 1.23 ± 0.03 (7.8 ± 0.2) × 10³ L7ep-11 17.1 ± 0.2 1.21 ± 0.03 (1.42 ± 0.04) × 10⁴ L7ep-12 5.74 ± 0.08 0.50 ± 0.02 (7.8 ± 0.2) × 10³ L72p-2c 16.1 ± 0.6  1.6 ± 0.1 (9.8 ± 0.8) × 10³ L7ep-2d   94 ± 3  1.7 ± 01 (5.4 ± 0.3) × 10⁴ L7ep-2e   44 ± 2 1.24 ± 0.09 (3.6 ± 0.3) × 10⁴ L7ep-2f   80 ± 2 1.58 ± 0.08 (5.0 ± 0.3) × 10⁴ L7ep-2g   80 ± 2 1.58 ± 0.08 (5.3 ± 0.4) × 10⁴ L7ep-2h   82 ± 2 0.94 ± 0.05 (8.7 ± 0.3) × 10⁴ L7ep-2i   44 ± 1 0.88 ± 0.04 (5.0 ± 0.3) × 10⁴ L7ep-2j   31 ± 1  0.8 ± 0.05 (4.0 ± 0.3) × 10⁴ L7ep-3c 35.2 ± 0.5 0.79 ± 0.02 (4.5 ± 0.1) × 10⁴ L73p-3d 25.2 ± 0.5 0.58 ± 0.03 (4.4 ± 0.2) × 10⁴

Example 9

Construction of Targeted Error-Prone Library. The CVQFL variant was used as the parent for the construction of an error-prone library with an average of six mutations per gene, targeted exclusively to Loop-7 of PTE (residues 253-276). The amino acid residue numbering of the sequence including the leader sequence has been retained. Approximately 4000 colonies from this library were screened with DEVX and a total of 12 variants were identified as being more active than the parent, CVQFL. The values of k_(cat)/K_(m) for the best variants, L7ep-1, L7ep-2 and L7ep-3, were improved 27-, 63-, and 36-fold, respectively, for the hydrolysis of DEVX.

The variant L7ep-2 (CVQFL+H254R/N265D/A270D/L272M/S276T) has 5 amino acid changes to the sequence of Loop-7, relative to the parent. These five sites, and residue positions 257 and 274, were subjected to further optimization. Two, two-site libraries (R254X/F257X, and M272X/I274X) and three, single-site libraries (D265X, D270X, and T276X) were constructed to ensure that the optimum amino acid residue is represented at each position. Screening the libraries with DEVX revealed no improvements at residue positions 254, 257, 265, or 270, but numerous improved combinations were identified in the 272X/274X library. One of these variants, L7ep-2a (L7ep-2+I274T), has a k_(cat) of 135 s⁻¹ and a k_(cat)/K_(m) 78-fold improved over wild type enzyme. To further optimize the L7ep-3 variant (CVQFL+H257Y/A270V/L272M), Loop-7 was subjected to a second round of targeted error-prone PCR. Screening with DEVX identified two variants, L7ep-3a (L7ep-3+I274N) and L7ep-3b (L7ep-3+A270D) that were substantially improved over the parent enzyme. Similar experiments were attempted using L7ep-2 as the starting template, but no improved variants were identified. The kinetic constants for the hydrolysis of DEVX by these mutants are presented in Table 2 and Table 3.

Example 10

Stereoselectivity of PTE Variants for Chiral VX Analogues. In this investigation there was no attempt to include a stereochemical preference in the screening of mutant libraries. Wild-type PTE is known to have a slight preference for the S_(P)-enantiomer of the VX chiral center.(18) To determine that there were no perturbations in stereo selectivity, the variants with improved catalytic activity against DEVX were analyzed using the chromophoric analogues R_(P)-1 and S_(P)-1, and the results are presented in Table 2. With the exception of L7ep-2, L7ep-2a, and L7ep-2b, the evolved variants have values of k_(cat)/K_(m) that are greater for the S_(P)-enantiomer than for the R_(P)-enantiomer.

Example 11

Enzymatic Specificity. To assess changes in substrate specificity, the enzyme variants were tested with paraoxon and demeton-S as alternative substrates. The results are provided in Table 4. The variants from the active site evolution experiments maintain a high enzymatic efficiency for paraoxon, although it is reduced nearly an order of magnitude from wild-type enzyme. The catalytic activity using demeton-S did not show any significant improvement for most of the variants tested. The exceptions are L7ep-2, L7ep-2a, and L7ep-2b, which have increased k_(cat) and decreased K_(m) values for demeton-S.

TABLE 4 Kinetic parameters for PTE variants with paraoxon and demeton-S^(a). Paroxon Demeton-S k_(cat) K_(m) k_(cat)/K_(m) k_(cat) K_(m) k_(cat)/K_(m) Variant (s⁻¹) (μM) (M⁻¹s⁻¹) (s⁻¹) (mM) (M⁻¹s⁻¹) WT 6700 100 6.7 × 10⁷ 1.4 1.2 1.1 × 10³ QF 41 5.3 7.7 × 10⁶ 6.3 2.6 2.7 × 10³ LQF 72 11.1 6.5 × 10⁶ 4.4 3.3 1.3 × 10³ VQF 108 10.5 1.0 × 10⁷ 10 6.1 1.7 × 10³ LQFL 90 11 8.2 × 10⁶ 5.2 3.1 1.7 × 10³ VQFL 66 5.4 1.2 × 10⁷ 4.2 3.9 1.1 × 10³ CVQFL 38 5.6 6.8 × 10⁶ 6.1 2.5 2.4 × 10³ VRN-VQFL 116 8 1.5 × 10⁷ 7.1 2.8 2.5 × 10³ VRNGS-VQFL 227 8.5 2.7 × 10⁷ 6.8 3.1 2.2 × 10³ L7ep-1 1590 116 1.4 × 10⁷ 0.12 1.0 1.2 × 10² L7ep-2 245 93 2.6 × 10⁶ 73 0.84 8.7 × 10⁴ L7ep-3 146 11.2 1.3 × 10⁷ 3.4 2.4 1.4 × 10³ L7ep-2a 243 46 5.3 × 10⁶ 32 0.58 5.4 × 10⁴ L7ep-2b 280 13.5 2.1 × 10⁷ 53 0.57 9.2 × 10⁴ L7ep-3a 85 7.2 1.2 × 10⁷ 1.8 2.5 7.4 × 10² ^(a)Standard errors from fits of the data fit to equation 1 are less than 10% of the stated values

Example 12

Hydrolysis of Racemic VX. Wild-type PTE and selected variants were characterized using racemic VX as a substrate and the results are presented in Table 5. Wild-type PTE has a low k_(cat) (0.9 s⁻¹) and relatively high K_(m), resulting in a diminished k_(cat)/K_(m) for the hydrolysis of VX. The variant QF dramatically improves both k_(cat) and K_(m) values resulting in a 100-fold increase in k_(cat)/K_(m). The VRN-VQFL variant had the highest value of k_(cat)/K_(m) that was increased more than 230-fold over wild-type enzyme. VRN-VQFL includes the following mutations A80V, K185R, I274N, F132V, H254Q, H257F, and S308L. The L7ep-3a had the highest k_(cat) and was increased more than 150-fold, relative to wild-type PTE. The QF mutant was shown to preferentially hydrolyze the S_(P)-enantiomer of VX by polarimetry.

TABLE 5 Activity of PTE variants with racemic VX^(a). Stereo- k_(cat)/K_(m) chemical Variant k_(cat) (s⁻¹) K_(m) (mM) (M⁻¹s⁻¹) Preference^(b) WT 0.9 ± 0.1 2.9 ± 0.9 3 ± 1 × 10² ND^(c) QF 16 ± 1 0.5 ± 0.1 3.0 ± 0.6 × 10⁴ 12:1 (S_(P)) CVQFL 45 ± 6 2.1 ± 0.7 2.2 ± 0.8 × 10⁴ 1:1 VRN-VQFL 44 ± 1 0.59 ± 0.09 7 ± 1 × 10⁴ 3:1 L7ep-1 11 ± 1 0.8 ± 0.2 1.4 ± 0.3 × 10⁴ ND L7ep-2 25 ± 2 1.3 ± 0.3 2.2 ± 0.3 × 10⁴ 5:1 L7ep-3 31 ± 2 0.5 ± 0.2 6 ± 2 × 10⁴ 4:1 L7ep-2a 56 ± 4 3.4 ± 0.7 1.6 ± 0.4 × 10⁴ 4:1 L7ep-2b 56 ± 14 8 ± 3 7 ± 4 × 10³ 12:1 (R_(P)) L7ep-3a 137 ± 22 5 ± 2 3 ± 1 × 10⁴ 4:1 ^(a)Standard errors from fits of the data to equation 1. ^(b)Identity of preferred enantiomer was not determined for variants with less than a 10-fold preference. ^(c)ND = not determined.

Stereoselective hydrolysis of racemic VX by the PTE mutants was evaluated by analyzing the time courses for the complete hydrolysis of VX at concentrations below the Michaelis constant. The presence of stereoselectivity in these time courses is manifested as the appearance of two exponential phases as observed with the QF variant where the ratio of rate constants is 12:1 (FIG. 5A).

FIG. 5. Representative time courses for the complete hydrolysis of racemic VX by selected PTE variants. (A) QF; (B) WT; (C) VRN-VQFL; (D) L7ep-3a (E) L7ep-2b; and (F) L7ep-2b and QF. The time courses for panels B and F were fit to equation 2, while the data for panels A, C, D, and E were fit to equation 3.

The CVQFL variant exhibited no selectivity (FIG. 5B), whereas the variants VRN-VQFL (3:1) and L7ep-3a (4:1) displayed relatively low selectivity (FIGS. 2C and 2D). For the L7ep-2b mutant, the observed stereoselectivity was 12:1 (FIG. 5E). The enantiomeric specificity of the L7ep-2b variant was determined by its ability to complement the hydrolysis of the slower R_(P)-enantiomer of VX after the addition of the variant QF. Plots of the fractional hydrolysis of VX as a function of time give two well-defined phases for each of these two variants (FIG. 5A and FIG. 5E). Mixing the two variants together resulted in a single well-defined monophasic curve demonstrating that the two variants prefer the opposite enantiomers (FIG. 5F). Therefore, the L7ep-2b variant preferentially hydrolyzes the R_(p)-enantiomer of VX. The ratios of rate constants for the L7ep-2, L7ep-3, and L7ep-2a mutants were 5:1, 4:1, and 4:1, respectively (Table 5). In the absence of enantiomerically pure VX, the modest selectivities for these variants prevented the definitive assignment of the preferred enantiomer.

Example 13

Construction of Active Site libraries by Overlap Extension. Mutagenic primers contained an NNS codon at the position of interest and extended 15 bp to either side of this codon. The PTE gene was amplified in three segments using standard PCR techniques (10 ng template and 125 ng each primer in a 50 μL reaction using pfuTurbo polymerase). The first segment extended from the 5′ end of the gene to 15 bp beyond the first mutagenic position. The second segment extended from 15 bp upstream of the first mutagenic position to 15 bp downstream of the second mutagenic position. The third segment extended from 15 bp upstream of the second mutagenic site to the 3′ end of the gene. The 5′ and 3′ primers included NdeI and EcoRI restriction sites respectively. A second PCR reaction was performed using the generated segments as the template DNA. The three fragments were combined in equimolar ratio (500 ng total) and amplified for 30 cycles with pfuTurbo using the primers for the 5′ and 3′ ends of the PTE gene. The overlaps between the fragments allowed for the formation of a single product corresponding to the size of the complete PTE gene. The product and vector were then digested with NdeI and EcoRI, gel purified and ligated together.

Example 14

Construction of Error Prone Library. Primer pairs used to amplify Loop-7 corresponding to the DNA sequence for residues 242-252 and 277-287. The reaction contained 20 ng template (CVQFL variant), 1 μM forward and reverse primers, 0.35 mM dATP, 0.4 mM dCTP, 0.2 mM dGTP, 1.35 mM dTTP, 1 mM MgCl₂, 1× GoGreen Taq Buffer (Promega, Madison Wis.) 1.5 mM MnCl₂ and 1 μL Go Taq in 50 μL reaction. Thermocycler program was 2 min initial denaturation at 95° C., followed by 30 cycles of 95° C. for 45 s, 60° C. for 1 min, 72° C. for 3 min, and a final elongation at 72° C. for 10 min. The remaining portions of the PTE gene were amplified using standard PCR techniques with the reverse primers for the Loop-7 fragment and the 5′ and 3′ end primer, resulting in three overlapping fragments. The final gene product was constructed by the overlap extension technique as described above. The mutated gene was digested with NdeI and EcoRI and ligated into pET 20 b (40 μL reaction containing 60 ng vector DNA, 3× molecular excess of PTE gene product, 4 μL T4 DNA ligase buffer and 2 μL T4 DNA ligase (NEB). Sequencing confirmed an average of 6 base pair changes per gene in loop-7. The identities of mutants from this library are given in Table 3.

Example 15

Enzyme Expression and Purification. BL21 (DE3) cells containing plasmid with wild-type or variant PTE were grown for ˜8 hours in 5 mL LB broth. 1 L cultures of Terrific Broth (12 g Tryptone, 24 g yeast extract, 4 mL glycerol, 2.3 g KH₂PO₄, 12.5 g K₂HPO₄ in 1 L H₂0) supplemented with 1.0 mM CoCl₂ were inoculated with 1 mL of the growing culture. Cells were grown overnight at 30° C. with shaking. Protein expression was induced by addition of 1.0 mM IPTG and expression proceeded for an additional 24 hours. Cells were harvested by centrifugation at 11,000 g for 10 minutes. Cell pellets were stored at −80° C. prior to use. Cells from 1 L of culture were resuspended in 100 mL purification buffer (50 mM HEPES (pH 8.5), 100 μM CoCl₂). Cellular lysis was achieved by sonication on ice for a total of 20 minutes using a medium power setting. Cell debris was removed by centrifugation at 18,500 g for 10 minutes. Protamine sulfate (0.45 g in 20 mL purification buffer) was added dropwise and incubated for 20 minutes to remove nucleic acids. Precipitated materials were removed by centrifugation at 18,500 g for 10 minutes. Supernatant was brought to 60% saturation with ammonium sulfate and stirred in the cold for 30 minutes to precipitate PTE. Protein was removed from the supernatant by centrifugation at 18,500 g for 20 minutes. The supernatant was decanted and the pellet re-dissolved in 5 mL purification buffer. Up to 5 mL of the protein solution was loaded on a Superdex 200 (16/60) preparatory size exclusion column on a GE Health Care (Piscataway, N.J.) AKTA FLPC system. Peak fractions were collected and assayed for activity against paraoxon. Fractions with the most activity were further purified using a gravity-fed DEAE column pre-equilibrated in purification buffer.

Example 16

Synthesis of DEVX. DEVX was made by the reaction of diethylchlorophosphate with N,N-diisopropylaminoethanthiol. 1.5 grams of N,N-diisopropylaminoethanthiol was added to 100 mL diethyl ether and cooled in a dry ice acetone bath and purged with N₂ gas. To this mixture, 7.5 ml of a 2.5 M solution of butyryl lithium in hexane was added. 1.5 g of diethylchlorophosphate was mixed with 30 mL diethyl ether in a separate flask purged with N₂ and cooled in a dry ice acetone bath. The cooled diethylchlorophosphate solution was then added to the thiol solution and the reaction stirred at room temperature for 3 hr. The reaction was then brought to 400 mL with ethyl ether and extracted with water to remove side products. Product was then extracted into the aqueous phase with 0.5 M HCl and ethyl acetate. The aqueous phase was neutralized with sodium bicarbonate and extracted with chloroform. The organic phase was dried over MgSO₄ filtered and evaporated yielding the desired product as a pure oil.

¹H NMR (300 MHz, CDCl₃): 4.05-4.174 (4H, m, OCH₂CH₃), 3.20-2.50 (6H, m, SCH₂CH₂N(CH)₂),

1.41-1.36 (6H, t, J=6.9 Hz, OCH₂CH₃), 1.05-1.03 (12H, d, J=4.8 Hz, CH(CH₃)₂

³¹P NMR (121.4 MHz CDCl₃): 29.77 ppm.

Example 17

Purification of racemic VX. VX samples were Chemical Agent Standard Analytical Reference Material (CASARM) and were of the highest purity available, typically 99.9+/−5.4 weight % by oxidation—reduction titration, traceable to National Institute of Standards and Technology through 0.1 N iodine solution SRM 136e. However, as received, the VX gave high background readings at 412 nm at the concentrations required for kinetic analysis and therefore required further purification as follows: 80.1 μL neat VX was added to 120 μL isopropyl alcohol (to aid in dissolution), then added to 800 μL of 3 mM DTNB in 50 mM HEPES, pH 8.0. To this solution was added approximately 1 gram of Dowex® 1×4 chloride form beads (Sigma-Aldrich) and agitated gently for several minutes until the beads turned red. The VX was subsequently decanted and added to more beads until essentially all the yellow color was removed to the beads and the VX solution was almost colorless. A standard curve was then generated using 6, 30, 60 and 96 μM dilutions of VX, reacted to completion enzymatically. VX concentration in the bead-treated solution was determined by linear regression analysis using the standard curve from the direct dilutions of VX.

Example 18

NMR Data Acquisition: All spectra were recorded on non-spinning samples at 25±2° C. with a Varian Unity INOVA 600 spectrometer (600 MHz ¹H operating frequency) fitted with a triple resonance, z-gradient probe. Routine ¹H free induction decay (FID) data sets of 16,384 complex points were collected as summations of eight or 16 acquisitions recorded with 10 ppm spectral windows, 90° pulse widths of 12 μsec, and 2 sec relaxation delays before archiving to computer disk. FID data sets were apodized with a line broadening factor of 0.3 Hz before Fourier transformation into spectra, manual phase correction into pure absorption mode, and chemical shift referencing to external tetramethylsilane.

³¹P FID data sets of 65,536 complex points were collected as summations of 32 acquisitions using 100 ppm spectral windows and 90° pulse widths of 30 μsec. All ³¹P data acquisitions incorporated inverse-gated 1H decoupling (decoupling only during FID acquisition) with a low power composite pulse sequence to increase signal-to-noise ratios without signal enhancements from ¹H-³¹P nuclear Overhauser effects.(31) Spin-lattice relaxation times (T1) for the VX ³¹P signal and that for the O-ethyl methylphosphonate (EMP) hydrolysis product were measured with the inversion recovery pulse sequence [180°-τ-90°-acquisition] incorporating nine randomized T delays. For quantitative ³¹P spectra, data sets were collected with relaxation delays>5T1 for all ³¹P signals in the spectra (˜12 sec) to allow complete signal relaxation, and the spectrometer carrier frequency was centered between the VX substrate signal (ca. 57 ppm) and that of the O-ethyl,methylphosphonate (EMP) hydrolysis product (ca. 23 ppm) to minimize off-resonance effects. The ³¹P{¹H} (¹H decoupled, ³¹P observe) data sets were apodized with a 5 Hz line broadening factor before Fourier transformation into spectra and manual phase correction into pure absorption mode. ³¹P chemical shift values in spectra were referenced to external 85% phosphoric acid at −0.73 ppm.(32)

Example 19

NMR Observation of Enzymatic Hydrolysis of VX: The enzymatic hydrolysis of VX in the presence of PTE enzymes was observed by using NMR spectroscopy to follow VX disappearance, or the appearance of its EMP hydrolysis product, over time. Enzymatic reactions were initiated by adding 0.1-25.0 μL of a single enzyme solution to a 1 mL aliquot of a racemic VX solution and briefly mixing before transferring to a NMR sample tube. This was immediately placed into the NMR spectrometer, and quantitative ³¹P{¹H} FID data sets were acquired at 7.5 min time intervals over 20-75 min. Enzymatic hydrolysis rates were calculated directly from the integral values of the quantitative ³¹P{¹H} signals, and included subtraction of the measured spontaneous rate (˜55 mole hr⁻¹) determined in separate experiments. The VX signal intensity decreases throughout the entire time course of the experiment until 75.0 min., where ≧99% of the intensity has disappeared (FIG. 8). EMP signal intensity increases over this same time frame, and at 75 min., it is the only signal observed in the spectrum.

Oligonucleotide pairs that contained the mutated codons at the specified sites were used as primers to amplify the genes for the wild-type enzyme and the following mutant enzymes: QF, YT, and GWT. The identities of the mutants are listed in Table 6. The mutations were added to each template sequentially to make the following mutant proteins: RN, QFRN, YTRN, GWT-d1, and GWT-d2.

TABLE 6 Identification of Mutants Abbreviation Mutations RN K185R/I274N QF H254Q/H257F GWT H254G/H257W/L303T QF-RN H254Q/H257F/K185R/I274N YT-RN H257Y/L303T/K185R/I274N GWT-d1 H254G/H257W/L303T/K185R/I274N GWT-d2 H254G/H257W/L303T/K185R/I274N/A80V GWT-d3 H254G/H257W/L303T/K185R/I274N/A80V/S61T GWT-f1 H254G/H257W/L303T/M317L/K185R/I274N GWT-f2 H254G/H257W/L303T/M317L GWT-f3 H254G/H257W/L303T/M317L/I106C/F132I/L271I/ K185R/I274N GWT-f4 H254G/H257W/L303T/M317L/I106C/F132I/L271I/ K185R/I274N/A80V GWT-f5 H254G/H257W/L303T/M317L/I106C/F132I/L271I/ K185R/I274N/A80V/R67H

Example 20

The multisite partially randomized PTE library was constructed by combining five separate segments of the gene for PTE as illustrated in FIG. 9 using primerless PCR for 15 cycles and then amplified by PCR for 55 cycles using primers specific for the 5′ and 3′ termini. The potential size of this multisite library is 1.9×10⁵ variants. The numbers below the residue identifier indicate the number of amino acids that were allowed during the construction of the library. The amplified PTE library was digested with NdeI and Avr II restriction enzymes and ligated into the GpdQ-pETDuet plasmid using T4 DNA ligase. The ligation mixture was purified using the QIAquick Kit (Qiagen) and then transformed into freshly made E. coli Top 10 competent cells (Life Technologies). The transformants were incubated at 37° C. for 1 hour and then plated on Luria-Bertani ampicillin agarose. Approximately 5.7×10⁵ colony forming units were collected and grown in LB medium for 6 hours at 37° C. The plasmids from the PTE library were extracted using the Promega Wizard Plus Miniprep Kit.

Example 21

Mutant libraries were constructed using GWT-d1 as the starting template to identify more active PTE variants for the hydrolysis of S_(P)-5. Nine amino acid residues in the substrate binding pocket were considered as potential “hot spots” for the construction of these PTE libraries. The single substitution library M317X was constructed first, followed by four double substitution libraries (W131X/F132X, F306X/Y309X, S308X/Y309X, and I106X/Y308X). Approximately 60 colonies from the M317X library and around 550 colonies from each of the double-substitution libraries were picked and subsequently screened with S_(P)-5. The variants of GWT with catalytic activities higher than background from the first round of screening were isolated and then rescreened with the same substrate. (Table 6). No improvement in the hydrolysis of S_(P)-5 (FIG. 4F) was found in the double-substitution libraries, W131X/F132X, F306X/Y309X, S308X/Y309X, and I106X/Y308X. FIG. 10 illustrates the screening of the M317X single-substitution library. The bars represent the relative catalytic activities of the GWT-d1, GWT-f1, and GWT-d1-M317F mutants as labeled. Those mutants represented by the unlabeled bars were not characterized or sequenced. The best mutant identified in this screen contained a leucine substitution for Met-317 and is denoted GWT-f1. FIG. 10 depicts the screening of the M317X mutant library against S_(P)-5 using GWT-d1 as the parental template. The bars represent the relative catalytic activities of the GWT-d1, GWT-d1-M317F mutants, respectively.

Example 22

The GWT-f1 mutant was partially randomized at six sites simultaneously. The total library contained 1.9×10⁵ potential variants. Eight colonies from this library were selected to verify that the targeted sites were randomized. The PTE/GpdQ-pETDuet plasmid library was transformed into E. coli BL21(DE3) cells. Approximately 5.8×10⁵ CFU were plated on phosphate-free minimal medium with 1 mM S_(p)-5 as the sole phosphorus source. The colonies that contained beneficial mutations for the hydrolysis of S_(P)-5 were identified as being larger in size than a background colony of the parent GWT-f1 mutant. Approximately 30 of these colonies were selected for growth in 96-well blocks and subsequently assayed for catalytic activity with S_(P)-5. The screening of the partially randomized multisite library with S_(P)-5 is shown in FIG. 11A. The first nine samples include the empty vector control, wild-type PTE, and the GWT-f1 parent. A single variant was found to have more activity than the GWT-f1 parent. This mutant (GWT-f3) contained three additional changes in the amino acid sequence: I106C, F1321, and L2711. The A80V mutation was added to the GWT-f3 mutant to create the GWT-f4 variant.

In FIG. 11A, screening of the six-site randomized library using GWT-f1 as the parental template with S_(P)-5. The bars represent the relative catalytic activities of the GWT-f1 and GWT-f3 mutants as labeled.

The GWT-f4 mutant served as the template for error-prone PCR (epPCR). Random mutagenesis of the GWT-f4 gene was conducted using the Mutazyme II DNA polymerase. Ten colonies from this library were selected to establish an average mutation rate of ˜1.5 mutations/1000 bp. The epPCR generated PTE/GpdQ-pETDuet library was transformed into E. coli BL21(DE3). Approximately 6×10⁵ CFU were plated on phosphate-free minimal medium plates with 1 mM S_(P)-5 as the sole phosphorus source. Colonies larger in size than the parental strain (GWT-f4) were assayed with S_(P)-5, and the results are shown in FIG. 11B. The first 20 samples include the empty vector, wild-type PTE, GWT-f3, GWT-f3-G129D, GWT-f3-I288F, and GWT-f3-H254W. The new variant, GWT-f5, contained a single mutation, relative to GWT-f4, at Arg-67 with a change to histidine.

In FIG. 11B, screening of the error-prone PCR library using GWT-f4 as the parental template with S_(P)-5. The bars represent the relative catalytic activities of the GWT-f4, GWT-f4-G129D, GWT-f4-I228F, GWT-f4-G254W, and GWT-f5 mutants as labeled.

Example 23

The outline for the discovery of PTE variants with enhanced activity for the hydrolysis of the S_(P)S_(C)-4 and S_(P)-5 (FIGS. 4D and 4F) by directed evolution is depicted in FIG. 12.

The structural modifications to GWT within the substrate binding pocket, surface and dimer interface have substantially enhanced substrate binding and catalytic turnover. The changes in the k_(cat)/K_(m) values of the S_(P)-enantiomers of the organophosphonates are depicted in FIG. 13A-13F.

Kinetic constants for sarin (GB), soman (GD), and cyclosarin (GF) were determined by monitoring the release of free fluoride at 25° C. in 50 mM bis-tris-propane buffer (pH 7.2) using a fluoride electrode. Stereospecificity for hydrolysis of nerve agents was obtained by following the complete hydrolysis of 0.5 mM racemic mixtures of GB or GF. Reactions were conducted in 50 mM bis-tris-propane buffer (pH 7.2) and followed by the release of fluoride.

Example 24

Screening and Kinetic Analysis of Wild-Type and Mutant Enzymes on GB, GD, and GF. For the purposes of initial screening, specific activities were determined with 3 mM substrate (Table 7). The YT mutant was very active with all three substrates, and the YT-RN mutant had higher activity than the wild type with GD. Therefore, kinetic constants were determined for these enzyme-substrate combinations (Table 8). The stereospecificity of variants was determined by following the fluoride released during the complete hydrolysis of GB or GF using the 0.5 mM racemic substrate. Substantial differences in the rates for the individual enantiomers result in biphasic curves. The specificity of GWT toward GF is known from polarimetry experiments,(9) while the stereopreference of the remaining variants was determined by the ability of the variant to complement the slow phase in the GWT-catalyzed reaction (Table 7). YT has the same stereopreference as GWT for GF and has previously been shown to have the same preference as GWT for GD.(5) The stereopreference for the variants toward GB was determined by the ability to complement the slow phase in the YT-catalyzed reaction (Table 7). Adding mutations to the variants YT and YT-RN will likely provide variants that have improved activity with G-agents over wild-type PTE. Mutations at various locations within the sequence of the YT mutant will be added and their activity measured to identify variants that exhibit high activity with G-agents. Such variants would be useful in the decontamination of people, items, and locations contaminated with one or more G-agents. In an embodiment, further improvements in catalytic activity could be gained by simultaneously mutating pairs of residues in the active site. In an embodiment, error-prone PCR could be utilized to obtain mutations within PTE. In an embodiment, mutations within the active site of PTE could provide increased catalytic activity toward a G-agent. In an embodiment, methods disclosed regarding mutating PTE and determining activity with V-agents can also be utilized with mutating PTE and determining activity with G-agents.

TABLE 7 Activity of Wild-Type and Mutant Enzymes with Racemic G-Agents* GB** GF** preferred preferred Enzyme GB GD GF enantiomer enantiomer WT 303  14 363 NA*** R_(P) YT 843 212 240 S_(P) S_(P) YT-RN 263 115 116 S_(P) S_(P) QF-RN  32  1.0  41 NA*** NA*** GWT  20  2.0  44 S_(P) S_(P) GWT-d1  57  2.0  7 S_(P) S_(P) GWT-d2  52  1.0 211 S_(P) S_(P) GWT-d3  48  8  35 S_(P) S_(P) GWT-f3 142  10  94 S_(P) S_(P) GWT-f5 240  19  59 S_(P) S_(P) *In micromoles per minute per milligram of protein. **Determined with 0.5 mM racemic substrate. ***No significant stereopreference under these conditions.

TABLE 8 Kinetic Constants for Hydrolysis of GB, GD, and GF* k_(cat)/K_(m) Enzyme substrate k_(cat) (s⁻¹) K_(m) (μM) (M⁻¹ s⁻¹) WT GB 430 ± 50 1800 ± 400 2.4 (0.6) × 10⁵ WT GD 12 ± 1  800 ± 200 1.5 (0.4) × 10⁴ WT GF 210 ± 30  900 ± 300 2.3 (0.8) × 10⁵ YT GB 520 ± 30 260 ± 50 2.0 (0.4) × 10⁶ YT GD 240 ± 20 460 ± 90 5 (1) × 10⁵ YT GF 130 ± 10 170 ± 50 8 (2) × 10⁵ YTRN GD 100 ± 10  300 ± 100 4 (2) × 10⁵ *Racemic mixtures of GB, GD, and GF were used for these measurements.

The kinetic parameters of the purified wild-type PTE and its mutants with the entire set of chiral organophosphonate compounds shown in FIGS. 4A-4L are provided in Tables 7, 9, and 10.

TABLE 9 Values of k_(cat) (s⁻¹) for Wild-Type PTE and Its Mutants* GWT- GWT- GWT- GWT- GWT- GWT- GWT- GWT- WT QF YT RN QFRN YTRN WT d1 d2 d3 f1 f2 f3 f4 f5 R_(P)-1 1.5e2 1.7e2 7.3e0 9.0e1 2.0e2 1.2e1 1.4e1 1.4e1 1.3e1 9.6e0 1.3e1 2.2e2 7.9e1 ND ND S_(P)-1 6.7e2 3.2e1 4.1e2 8.2e2 4.5e1 1.0e3 1.9e2 2.9e2 5.3e2 4.0e2 3.6e2 4.4e2 6.6e2 1.1e3 7.2e2 R_(P)-2 1.0e2 4.8e1 1.8e1 6.6e1 6.6e1 2.0e1 ND 2.1e1 2.2e1 5.9e1 9.8e0 3.3e1 ND ND ND S_(P)-2 4.0e1 7.2e0 3.7e2 2.0e1 1.1e1 7.0e2 9.2e1 8.6e1 1.3e2 2.0e2 3.0e2 2.3e2 6.2e2 1.1e3 5.9e2 R_(P)-3 9.3e1 7.0e1 5.1e1 4.8e1 1.3e2 4.3e1 2.0e1 8.0e0 1.3e1 2.2e1 2.9e1 3.4e1 1.3e1 1.5e1 ND S_(P)-3 2.2e1 6.3e0 1.0e2 1.6e1 1.3e1 7.7e2 5.0e1 5.5e1 5.8e1 6.0e1 8.0e1 8.8e1 1.4e2 2.5e2 1.8e2 R_(P)R_(C) 3.4e0 5.5e−1 4.1e−1 4.5e0 1.1e0 5.8e−1 2.0e0 2.4e0 4.3e0 ND 4.0e0 ND ND ND 2.9e0 -4 R_(P)S_(C) 4.5e−1 1.7e−1 ND 4.2e−1 3.3e−1 1.9e0 2.1e−1 1.4e0 ND ND 8.9e−1 1.9e0 ND ND 1.9e0 -4 S_(P)R_(C) 7.7e−1 6.3e−1 6.3e0 1.3e0 1.2e0 4.3e0 1.2e1 1.4e1 5.0e1 6.4e1 3.1e1 3.1e1 1.6e1 4.7e1 1.7e1 -4 S_(P)S_(C) 1.6e−2 3.3e−1 2.1e0 ND 5.e−1 3.2e0 2.9e0 6.5e0 1.2e1 2.4e1 5.7e1 8.1e0 4.2e0 5.6e0 6.1e0 -4 R_(P)-5 ND 3.8e1 5.9e0 2.5e1 2.2e1 1.7e1 8.1e−1 ND 9.7e−1 ND ND ND 2.2e0 ND 3.3e0 S_(P)-5 ND ND 5.1e0 1.3e−1 4.1e−1 7.2e0 1.9e1 3.1e0 4.7e1 4.4e1 2.6e1 3.1e1 4.4e1 1.2e2 1.2e2 *The standard errors, from fits of the data to v/E_(t) = (kcat[A]/(K_(m) + [A]), are less than 20% of the stated values. ND, not determined.

TABLE 10 Values of k_(cat)/K_(m) (M⁻¹ s⁻¹) for Wild-Type PTE and Its Mutants* QFR YTR GWT- GWT- GWT- GWT- GWT- GWT- GWT- GWT- WT QF YT RN N N GWT d1 d2 d3 f1 f2 f3 f4 f5 R_(P)-1 4.9e5 1.5e6 2.4e3 1.7e5 3.0e6 4.3e3 1.5e3 2.5e3 6.1e3 9.1e3 1.0e5 5.2e4 6.1e3 7.2e3 8.5e3 S_(P)-1 1.2e6 7.1e6 1.6e5 7.4e5 8.0e6 1.7e5 2.2e5 1.9e5 1.2e6 1.2e6 7.2e5 6.2e5 1.3e5 2.3e5 2.9e5 Rp-2 5.8e5 8.2e5 2.5e3 2.8e5 1.6e6 3.4e3 1.8e3 3.5e3 6.0e3 8.1e3 1.4e4 4.7e3 3.4e3 4.2e3 6.1e3 S_(P)-2 2.7e4 1.2e6 1.1e5 2.6e4 1.6e6 1.4e5 5.9e4 8.6e4 4.6e5 4.3e5 1.4e5 1.9e5 1.2e5 2.4e5 4.2e5 R_(P)-3 8.5e5 3.1e5 1.3e4 4.0e5 1.3e6 1.3e4 1.5e3 3.0e3 5.4e3 7.6e3 3.3e3 3.8e3 8.2e2 2.6e3 2.2e3 S_(P)-3 3.4e4 1.6e6 7.3e4 4.8e4 1.4e6 3.9e5 1.8e5 5.0e5 1.1e6 1.2e6 6.7e5 1.0e6 1.1e6 2.3e6 1.9e6 R_(P)R_(C)-4 1.3e3 1.9e2 5.8e1 3.0e3 2.8e2 3.0e2 2.2e2 6.8e2 6.4e2 5.6e2 4.2e2 4.1e2 6.3e2 7.9e2 8.5e2 R_(P)S_(C)-4 2.0e2 5.5e1 1.6e1 4.6e2 7.4e1 1.9e2 1.3e2 1.2e2 1.5e2 1.4e2 2.1e2 1.4e2 1.4e2 2.0e2 1.8e2 S_(P)R_(C)-4 1.1e2 1.6e3 1.8e3 2.3e2 1.8e3 1.2e3 8.1e3 2.3e4 6.0e4 8.7e4 1.3e4 1.4e4 3.2e3 5.0e3 3.8e3 S_(P)S_(C)-4 3.2e0 6.2e1 2.5e2 1.5e1 9.6e1 4.8e2 1.7e3 4.2e3 8.1e3 1.1e4 2.6e3 2.5e3 1.5e3 1.5e3 1.2e3 R_(P)-5 1.6e4 5.2e3 1.9e3 1.7e4 9.0e3 3.5e3 2.5e2 3.0e2 5.4e2 5.5e2 6.0e2 8.6e2 4.5e2 5.1e2 7.7e2 S_(P)-5 2.1e1 3.3e2 5.8e3 2.8e1 3.6e2 1.4e4 2.8e4 1.0e4 5.2e4 1.5e5 3.9e4 7.7e4 1.2e5 2.5e5 3.2e5 *The standard errors, from fits of the data to eq 1, are less than 20% of the stated values.

Example 25

Materials. Growth media and antibiotics were procured from Research Products Incorporated. DNA polymerase was obtained from Agilent. Other supplies for the molecular biology experiments were acquired from New England Biolabs. DEVX and N,N-diisopropylaminoethanethiol were synthesized as previously reported.(37, 44) The individual enantiomers of p-acetophenyl VR (APVR) were synthesized as previously reported.(39) Samples of VX and VR were Chemical Agent Standard Analytical Reference Material (CASARM) of the highest purity available, and were further purified as described previously.(37) Unless otherwise noted, all other chemicals were purchased from Sigma Aldrich. The organophosphorus nerve agents used in this investigation are highly toxic and should be used with the proper safety precautions. PTE: phosphotriesterase; DEVX: O,O-diethyl-VX; DMVX: O,O-dimethyl-VX; DEVR: O,O-diethyl-VR; and OMVR: O-methyl-VR.

Example 26

Synthesis of Dimethyl VX. Dimethyl VX (DMVX) was made by the reaction of dimethyl chlorophosphate with N,N-diisopropylaminoethanethiol. N,N-diisopropylaminoethanethiol (1.5 grams; 9.3 mmol) was added to 100 mL of diethyl ether and allowed to cool in a dry ice/acetone bath before being purged with N₂. To this mixture was added 7.5 mL (2.0 equivalents) of a 2.5 M solution of butyl lithium in hexanes and the reaction allowed to come to room temperature before re-cooling in a dry ice/acetone bath. Dimethyl chlorophosphate (2.0 g; 1.5 equivalents) was mixed with 30 mL of diethyl ether in a separate flask and cooled. The dimethyl chlorophosphate solution was then added to the thiol solution and the reaction stirred at room temperature for 3 hours. The reaction was brought to 400 mL with diethyl ether and extracted with water. The product was extracted into the aqueous phase with 0.5 M HCl. The aqueous phase was neutralized with sodium bicarbonate and extracted with dichloromethane. The organic phase was dried over Na₂SO₄, filtered, and evaporated to dryness. The product was further purified by silica gel chromatography. The product was dissolved in dichloromethane and eluted from the column using using a 0-5% step gradient of methanol in dichloromethane. Fractions containing the desired product were combined and the solvent evaporated to provide the product as an oil. Overall isolated yield was 8%. ¹H NMR (300 MHz, CDCl₃): 3.84-3.77 (6H, d, J=12.6 Hz, OCH₃), 3.08-2.62 (6H, m, SCH₂CH₂N(CH)₂), 1.05-0.98 (12H, d, J=6.9 Hz, CH(CH₃)₂. ³¹P NMR (121.4 MHz, CDCl₃): 32.74 ppm.

Example 27

Synthesis of Diethyl VR. Diethyl VR (DEVR) was made by the reaction of diethyl chlorophosphate with N,N-diethylaminoethanethiol. N,N-diethylaminoethanethiol was prepared from the hydrochloride salt by dissolving the compound in a saturated NaHCO₃ solution and extraction with diethyl ether. The organic phase was dried over Na₂SO₄ and evaporated in vacuo at room temperature. The remaining oil was distilled (50° C.) under high vacuum and recovered as a pure liquid in a dry ice cooled trap. N,N-diethylaminoethanethiol (1.1 grams; 8.35 mmol) was added to 100 mL of diethyl ether and cooled in a dry ice/acetone bath before being purged with N₂. To this mixture was added 10 mL (3.0 equivalents) of a 2.5 M solution of butyl lithium in hexanes and the reaction allowed to come to room temperature before re-cooling in a dry ice/acetone bath. Diethyl chlorophosphate (2.9 g; 2 equivalents) was mixed with 30 mL of diethyl ether in a separate flask, purged with N₂, and then cooled in a dry ice/acetone bath. The cooled diethyl chlorophosphate solution was added to the thiol solution and the reaction stirred at room temperature for 3 hours. The reaction was brought to 400 mL with diethyl ether and extracted with water. The product was extracted into the aqueous phase with 0.5 M HCl. The aqueous phase was neutralized with sodium bicarbonate and extracted with dichloromethane. The organic phase was dried over Na₂SO₄, filtered, and then evaporated, yielding the product as an oil. Further purification was conducted using silica gel chromatography as described above. Overall yield of the isolated product was 7%. ¹H NMR (300 MHz, CDCl₃): 4.27-4.10 (4H, m, OCH₂CH₃), 2.99-2.52 (8H, m, SCH₂CH₂N(CH₂)₂), 1.43-1.34 (6H, t, J=7.5 Hz, OCH₂CH₃), 1.11-1.01 (6H, t, J=7.2 Hz, CH₂CH₃). ³1P NMR (121.4 MHz, CDCl₃): 28.50 ppm.

Example 28

Synthesis of O-methyl VR. O-methyl VR (OMVR) was synthesized by the reaction of methyl isobutyl chlorophosphate with N,N-diethylaminoethanethiol. N,N-diethylaminoethanethiol was prepared from the hydrochloride salt as described above. Methyl isobutyl chlorophosphate was prepared by dissolving 750 μL (8.4 mmol) of isobutanol in 50 mL of diethyl ether. The atmosphere was purged with N₂ and then the mixture was chilled in a dry ice/acetone bath. A total of 3.3 mL (1.0 equivalent) of 2.5 M butyl lithium in hexanes and 1.5 g (1.0 equivalents) of methyl dichlorophosphate was added, and the reaction stirred for three hours at room temperature.

In a separate flask, 1.2 g (1.0 equivalents) of N,N-diethylaminoethanethiol was dissolved in 50 mL of diethyl ether and chilled in a dry ice/acetone bath. A total of 5 mL (1.5 equivalents) of 2.5 M butyl lithium was added and the reaction warmed to room temperature. The methyl isobutyl chlorophosphate and the thiol solutions were chilled in a dry ice/acetone bath and combined. The reaction was allowed to proceed at room temperature for 3 hours. The reaction was then brought to 400 mL with diethyl ether and washed with water. The product was extracted with 0.5 M HCl, neutralized with sodium bicarbonate, and then extracted with dichloromethane. The organic phase was dried over Na₂SO₄ and evaporated to yield the product as an oil. Overall yield of final product was 15%. ¹H NMR (300 MHz, CDCl₃): 3.92-3.72 (5H, m, OCH₂CH(CH₃)₂, OCH₃), 2.95-2.45 (8H, m, SCH₂CH₂N(CH₂)₂), 2.04-1.88 (¹H, OCH₂CH(CH₃)₂), 1.06-0.97 (6H, t, J=7.0 Hz, NCH₂CH₃), 0.97-0.90 (6H, d, J=6.8 Hz, OCH₂CH(CH₃)₂. ³¹P NMR (121.4 MHz CDCl₃): 30.30 ppm.

Example 29

Mutagenesis, Expression and Enzyme Purification. The gene for PTE was cloned into the expression vector pET 20b between the NdeI and EcoRI restriction sites as previously described.(39) The new variants of PTE were generated by introducing the mutations I106C, I106G, and L308S into the appropriate templates by site directed mutagenesis using the Quick Change (Agilent) protocol. DNA sequencing at the Gene Technologies Laboratory at Texas A&M University verified the specific mutations. The proteins were expressed and purified as previously described. (37) Briefly, the variants were freshly transformed into E. coli BL21 (DE3) cells by electroporation, and single colonies used to inoculate 5.0 mL cultures of LB medium. After 8 hours of growth at 37° C., 1.0 mL of this culture was used to inoculate 1 L cultures of Terrific Broth supplemented with 1.0 mM CoCl₂. The bacterial cultures were grown at 30° C. IPTG was added to a final concentration of 1.0 mM after 24 hours and growth continued for 40 hours. The cells were harvested by centrifugation and stored at −80° C. prior to purification. Cells were resuspended in 100 mL of purification buffer (50 mM HEPES, pH 8.5, with 100 μM CoCl₂) and then lysed by sonication. The cell debris was cleared by centrifugation, nucleic acids were precipitated by protamine sulfate (0.45 g in 20 mL purification buffer per liter of culture), and then removed by centrifugation. The PTE mutants were precipitated with ammonium sulfate (60% saturation) and recovered by centrifugation. The pellet was resuspended in ˜5 mL of purification buffer, filtered (0.45 μm) and loaded onto a GE Superdex 200 (16/60) preparatory size exclusion column using a BioRad NCG FPLC system. Fractions with catalytic activity for the hydrolysis of paraoxon were pooled and then eluted from a 3.0 g (dry weight) DEAE Sephadex A25 resin that was pre-equilibrated in purification buffer. Protein purity was verified by SDS-PAGE.

Generation and Characterization of New PTE Variants. The PTE variants QF, CVQFL, VRN-VQFL and L7ep-3a were previously shown as having substantially improved activity for the hydrolysis of VX.(37) The stereoselectivity of these mutants for the chiral center contained in VR was determined using the isolated enantiomers of APVR (Table 11). With the exception of QF, the VX-optimized variants of PTE prefer to hydrolyze the R_(P)-enantiomer of the chiral center for VR. The crystal structure of L7ep-3a suggests that the mutations I106C and S308L affect the size of the small-group pocket. In order for the S_(P)-enantiomer of VR to productively bind in the active site, the larger isobutyl group must be positioned in the small-group pocket of PTE. In an effort to maximize the hydrolysis of S_(P)-VR, a series of variants was created to change the substitutions made to residues 106 and 308 in the variants previously optimized for the hydrolysis of VX.

TABLE 11 Kinetic constants for PTE variants with APVR¹. R_(P)-APVR S_(P)-APVR k_(cat) K_(m) k_(cat)/K_(m) k_(cat) K_(m) k_(cat)/K_(m) Enzyme (s⁻¹) (mM) (M⁻¹s⁻¹) (s⁻¹) (mM) (M⁻¹s⁻¹) Ratio² Wild-type 84 1.7 4.9 × 10⁴ 25 4.5   6 × 10³ 8:1 R QF 57 0.36 1.6 × 10⁵ 8.7 0.030 2.9 × 10⁵ 1.8:1 S CVQFL 46 0.18 2.6 × 10⁵ 21 0.19 1.1 × 10⁵ 2.5:1 R CVQFL C106I* 50 0.15 3.3 × 10⁵ 14 1.5 9.5 × 10³ 35:1 R CVQFL-I106G 174 1.4 1.2 × 10⁵ 36 0.20 1.8 × 10⁵ 1.5:1 S CVQFL-L308S* 122 2.0 6.0 × 10⁴ 8.1 0.19 4.2 × 10⁴ 1.4:1 R CVQFL-I106G/L308S 100 4 2.4 × 10⁴ 40 0.24 1.6 × 10⁵ 6.7:1 S VRN-VQFL 55 0.16 3.4 × 10⁵ 29 1.7 1.7 × 10⁴ 20:1 R VRN-VQFL-I106C 72 0.23 3.2 × 10⁵ 33 0.23 1.4 × 10⁵ 2.3:1 R VRN-VQFL-I106G 56 0.41 1.4 × 10⁵ 159 0.18 9.0 × 10⁵ 6.6:1 S VRN-VQFL-L308S 17 0.52 3.2 × 10⁴ 5.0 0.13 3.9 × 10⁴ 1.2:1 S VRN-VQF-I106C/L308S 160 1.7 1.0 × 10⁵ 51 1.5 3.4 × 10⁴ 3:1 R VRN-VQFL-I106G/L308S 45 2.1 2.2 × 10⁴ 53 0.18 3.0 × 10⁵ 14:1 S L7ep-3a 101 0.62 1.6 × 10⁵ 56 0.5 1.1 × 10⁵ 1.5:1 R L7ep-3a I106G 58 0.71 8.2 × 10⁴ 166 0.31 5.3 × 10⁵ 6.5:1S *The mutations C106I and L308S are revertants back to the wild-type amino acid sequence. ¹Errors from curve fitting are less than 10% with the exception of CVQFL-I106G/L308S, which has an error of 20% due to the high K_(m) value. ²The ratio is k_(cat)/K_(m) values for fast enantiomer and slow enantiomer, with the preferred enantiomer identified.

Example 30

Enzymatic Activity. Catalytic activity with paraoxon was followed by monitoring the release of p-nitrophenol at 400 nm (ΔE400=17,000 M⁻¹ cm⁻¹) in 250 μL reaction volumes containing 50 mM CHES, pH 9.0, 100 μM CoCl₂, and 0-1.0 mM paraoxon. Activity with APVR utilized the same reaction conditions as paraoxon with the release of the leaving group monitored at 294 nm (Δ E294=7,710 M⁻¹ cm⁻¹). Activity with DEVX, DMVX, DEVR, and OMVR was measured in 250 μL reactions containing 50 mM HEPES, pH 8.0, 100 μM CoCl₂, 0.3 mM DTNB and 0-1.0 mM substrate. The release of the thiol leaving group was followed by inclusion of DTNB in the assay mixture (Δ E412=14,150 M⁻¹ s⁻¹). All assays were initiated by the addition of the appropriately diluted enzyme and monitored in a 96-well format using a Molecular Devices SpectraMax 364 Plus plate reader. Reactions were monitored for 15 minutes at 30° C. and the linear portion of the time course was used to calculate the initial rate. Kinetic constants were determined by fitting the data to the Michaelis-Menten equation.(45) When saturation could not be observed, the data was fit to a linear equation and the slope taken as k_(cat)/K_(m).

The catalytic activities of these variants were first characterized against the insecticide paraoxon and the V-agent analog DEVX (Table 12), and then the stereochemical preferences were determined using APVR (Table 11).

TABLE 12 Kinetic parameters for PTE variants with paraoxon and DEVX¹. Paraoxon DEVX k_(cat) K_(m) k_(cat)/K_(m) k_(cat) K_(m) k_(cat)/K_(m) Enzyme (s⁻¹) (uM) (M⁻¹s⁻¹) (s⁻¹) (mM) (M⁻¹s⁻¹) Wild-type 2230 81 2.8 × 10⁷ 1.1 0.87 1.2 × 10³ QF 41 5.3 7.7 × 10⁶ 6.1 1.4 4.2 × 10³ CVQFL 38 5.6 6.8 × 10⁶ 16 0.76 2.1 × 10⁴ CVQFL-C106I* 66 5.4 1.2 × 10⁷ 14 0.65 2.2 × 10⁴ CVQFL-L308S* 33 6.7 4.8 × 10⁶ 13 3.2 4.1 × 10³ CVQF-I106G/ 48 25 1.9 × 10⁶ nd nd 3.1 × 10² L308S CVQFL-C106I/ 108 11 1.0 × 10⁷ 19 1.0 1.9 × 10⁴ L308S CVQFL-I106G 456 22 2.0 × 10⁷ 31 2.8 1.1 × 10⁴ VRN-VQFL 116 8 1.5 × 10⁷ 22 0.73 3.1 × 10⁴ VRN-VQFL- 103 5.3 1.9 × 10⁷ 23 0.80 2.8 × 10⁴ I106C VRN-VQFL- 446 21 2.1 × 10⁷ nd nd 5.0 × 10³ I106G VRN-VQFL- 15 1.7 8.8 × 10⁶ 5.1 0.35 1.5 × 10⁴ L308S VRN-VQFL- 35 3.6 9.7 × 10⁶ 8.6 1.6 5.4 × 10³ I106C/L308S VRN-VQFL- 58 9.2 6.2 × 10⁶ nd nd 4.1 × 10² I106G/L308S L7ep-3a 142 7.2  1.2 × 10e⁷ 5 0.60 8.5 × 10⁴ L7ep-3a I106G 545 33 1.67 × 10⁷  nd nd 7.7 × 10³ *The mutations C106I and L308S are revertants to the wild-type amino acid sequence. ¹ Errors from curve fitting were less than 10%.

Inclusion of the I106C mutation substantially reduced the preference for the hydrolysis of the R_(P)-enantiomer, while it tended to have relatively little effect on the hydrolysis of DEVX. For example, the CVQFL variant has a 2.5-fold preference for the R_(P)-enantiomer of the VR chiral center, but CVQFL-C106I has a 35-fold preference for the R_(P)-enantiomer. Despite this large difference in stereoselectivity, both of these variants hydrolyze DEVX with a k_(cat)/K_(m) of ˜2×10⁴ M⁻¹ s⁻¹. The removal of the S308L mutation from the VX-optimized variants also results in a substantial diminished preference toward the R_(P)-enantiomer, but in most cases it also resulted in diminished activity against DEVX. VRN-VQFL prefers the R_(P)-enantiomer of APVR by 20-fold. The variant VRN-VQFL L308S has a preference of 1.2-fold, but the activity against DEVX was also diminished 2-fold. When glycine was substituted at position 106, the stereochemical preference shifted to the S_(P)-enantiomer of APVR. L7ep-3a prefers the R_(P)-enantiomer by 1.5-fold, but L7ep-3a I106G prefers the S_(P)-enantiomer by 6.5-fold. Unfortunately, the I106G mutation reduced the activity against DEVX by more than an order of magnitude in these variants.

Example 31

Stereoselelctive Hydrolysis of Racemic VX and VR. Low initial concentrations (19 to 160 μM) of racemic VX and VR were hydrolyzed by variants of PTE in a solution containing 0.1 mM CoCl₂, 0.3 mM DTNB, and 50 mM Bis-Tris-propane, pH 8.0. The reactions were followed to completion and the fraction hydrolyzed plotted as a function of time. The time courses were fit to equations 1 and 2 where F is the fraction hydrolyzed, a and b are the magnitudes of the exponential phases, t is time, and k₁ and k₂ are the rate constants for each phase.(39)

F=a(1−e ^(−k)1^(t))  (1)

F=a(1−e ^(−k)1^(t))+b(1−e ^(−k)1^(t))  (2)

Stereochemical preferences were determined using the previously described complementation method.(37) Briefly, variants with large stereoselective preferences were placed in a reaction with mutants of PTE of known stereoselective preferences under conditions where each variant alone would exhibit a similar rate for the first exponential phase. If the variants prefer the same enantiomer, the resulting time course will exhibit two distinct phases. If the variants have the opposite enantiomers as the preferential substrate, the time courses will exhibit a single exponential phase.

Catalytic Activity with VX and VR. The most promising new variants were tested with racemic VX and VR. The assays were conducted for the complete hydrolysis of a single low concentration of these agents to enable the observation of exponential time courses, corresponding to the hydrolysis of each enantiomer contained within the racemic mixture. The kinetic constants are presented in Table 13. For enzyme variants with large stereochemical preferences, the identity of the preferred enantiomer was determined by the ability of the variant to complement the slow phase of a variant of known preference. Wild-type PTE is known to prefer to hydrolyze the R_(P)-enantiomer of the VR chiral center, while QF is known to prefer the S_(P)-enantiomer of VX.(37, 39) None of the variants tested, with the exception of QF, exhibited large stereochemical preferences for hydrolysis of the two enantiomers of VX. Removal of the S308L mutation (VRN-VQFL L308S) resulted in a 2-fold reduction in catalytic activity for the faster enantiomer of VX and a 5-fold reduction in the rate of hydrolysis for the slower enantiomer. Introduction of the I106G mutation (VRN-VQFL-I106G) led to the complete hydrolysis of racemic VX without detectable selectivity, but at a rate 6-fold slower than VRN-VQFL had for the slower enantiomer.

TABLE 13 Kinetic constants with the racemic nerve agents VX and VR¹. VX VR k_(cat)/K_(m1) k_(cat)/K_(m2) k_(cat)/K_(m1) k_(cat)/K_(m2) Enzyme (M⁻¹s⁻¹) (M⁻¹s⁻¹) Ratio (M⁻¹s⁻¹) (M⁻¹s⁻¹) Ratio² Wild-type 8.4 × 10¹ nd 1.1 × 10² 4.3 × 10⁰ 25:1 R QF 1.7 × 10⁴ 1.5 × 10³  12:1 S 4.8 × 10² 7.9 × 10¹ 6:1 CVQFL 1.0 × 10⁵ 1:1 5.5 × 10³ 8.9 × 10² 6:1 VRN-VQFL 1.1 × 10⁵ 4.3 × 10⁴ 4:1 2.4 × 10³ nd >30:1 R VRN-VQFL-I106G 6.6 × 10³ 1:1 2.0 × 10³ 4.1 × 10² 5:1 VRN-VQFL-L308S* 6.2 × 10⁴ 8.9 × 10³ 7:1 2.7 × 10² 1:1 VRN-VQFL- 4.9 × 10³ 1.7 × 10³ 3:1 2.1 × 10³ 6.7 x 101 31:1 S I106G/L308S L7ep-3a 8.3 × 10⁵ 2.2 × 10⁵ 4:1 2.2 × 10³ 2.1 × 10² 10:1 L7ep-3a I106G 2.0 × 10⁴ 6.2 × 10³ 3:1 2.6 × 10³ 6.9 × 10² 3.8:1 *The mutation L308S is a revertant to the wild type amino acid sequence. ¹Errors from curve fitting are less than 5%. ²The ratio is k_(cat)/K_(m) values for fast enantiomer and slow enantiomer. If the preferred enantiomer is not listed it has not been determined.

With racemic VR, the VRN-VQFL variant exhibited a 20-fold enhancement in the rate of hydrolysis compared to the wild-type enzyme, but this mutant was found to only hydrolyze the relatively nontoxic R_(P)-enantiomer of VR. Removal of the S308L mutation (VRN-VQFL L308S) enabled the hydrolysis of both enantiomers of VR, with complete loss of stereoselectivity. This represents a 64-fold improvement toward the hydrolysis of the toxic S_(P)-enantiomer compared to wild-type PTE. The introduction of the I106G mutation in the VRN-VQFL-I106G/L308S variant resulted in a strong preference for the hydrolysis of the S_(P)-enantiomer relative to the R_(P)-enantiomer. VRN-VQFL-I106G, which has both the I106G and S308L mutations, has much less stereochemical preference, but the kinetic data for the hydrolysis of the two enantiomers of APVR indicate that the stereochemical preference is for the SP-enantiomer. The best variant identified for the hydrolysis of VR was L7ep-3a I106G, which has a k_(cat)/K_(m) of 2.6×103 M⁻¹ s⁻¹ for the faster enantiomer. While the stereoselectivity was not sufficient to determine the stereochemical preference with VR directly, the kinetic data with the two enantiomers of APVR has identified the preferred enantiomer as the highly toxic S_(P)-enatiomer. The L7ep-3a I106G mutant thus has a 620-fold enhanced rate of hydrolysis of S_(P)-VR relative to wild-type PTE.

Example 32

X-ray Crystallography. The PTE mutants L7ep-3a and L7ep-3a I106G were crystallized at 18° C. using the vapor diffusion method. In the crystallization experiments, 1.0 μL of protein (10 mg/mL with 1.0 mM CoCl₂) was mixed with 1.0 μL of the precipitant solution (100 mM sodium cacodylate pH 5.5-7.0, 0.2 M magnesium acetate, 15-30% PEG 8000), and then equilibrated against 500 μL of the same precipitant solution using Intelliplates. Protein crystals appeared within a week and grew to maximum dimensions (200 μm×15 μm×15 μm) after 21 days. Prior to data collection, the crystals were soaked for 30 seconds in a cryoprotectant solution of the mother liquor containing 30% ethylene glycol and then frozen in liquid nitrogen. Diffraction data were collected locally at 120 K on an R-AXIS IV detector with Cu Kα X-rays produced from a rotating anode generator. X-ray data reduction and scaling were performed with HKL2000.(46) Structures of the PTE mutants L7ep-3a and L7ep-3aG were determined by molecular replacement using the coordinates of wild type PTE (PDB id: 1DPM) as the search model. The structures were built using COOT and refined with simulated annealing, B-factor randomization, and coordinate shaking using PHENIX.(47, 48) Later stages of refinement were also done in PHENIX using individual coordinate, anisotropic B-factor, and occupancy optimization. The PTE mutant structures were refined with R_(work)/R_(free) values of 13.5-21.5% with excellent geometry (Table 14).

TABLE 14 X-ray crystallography data for L7ep-3a and L7ep-3a I106G. Variant L7ep-3a L7ep-3a I106G Resolution, Å (Highest 50.00-2.01  50.00-2.01  resolution shell) (2.04-2.01) (2.04-2.01) Space group P2₁ P2₁ Cell dimensions a 45.53 45.85 b 80.64 80.63 c 78.73 78.84 γ 106.60 106.94 R_(sym) 0.087 0.057 I/σI 13.2 (3.0) 18.9 (2.8) Completeness, % 98.3 (96.1) 95.8 (91.1) (Highest resolution shell) Redundancy 3.5 (3.2) 3.7 (3.2) (Highest resolution shell) Refinement Resolution, Å 29.61-2.01  29.57-2.01  No. of reflections 35,603 34,657 R_(work)/R_(free) 0.1574/0.2145 0.1348/0.1838 No. of nonhydrogen atoms Total 5420 5395 Water 383 384 B-factors Protein 27.56 28.08 Co²⁺ 30.72 30.60 Root mean square deviations Bond lengths, Å 0.006 0.007 Bond angles, ° 1.09 1.10 Ramachandran Favored, % 97.4 97.1 Allowed, % 2.6 2.9 Outliers, % 0 0

Three-Dimensional Structure of the PTE Mutant L7ep-3a. The PTE variant L7ep-3a has the highest reported k_(cat) for the hydrolysis of the nerve agent VX.(37) In an effort to elucidate the mechanism by which the activity of this mutant is enhanced, the enzyme was crystallized and the structure determined to a resolution of 2.01 Å by X-ray diffraction methods (PDB id: 4ZST). FIG. 16 depicts (A) Structural alignment between wild-type PTE (light) and L7ep-3a mutant (dark). Selective active site residues are labeled and shown. Loop-7 and -8 are shown. (B) Expanded view of Loop-7 and -8. Mutated residues and residues with significant structural perturbations are shown as sticks. The wild type structure is taken from PDB id: 1DPM and the L7ep-3a structure is taken from PDB id: 4ZST. The overall structure of L7ep-3a is very similar to wild-type PTE (FIG. 16A). The core of the (β/α)8-barrel matches very well between the two structures with a Cα RMSD of 0.64 Å. The only significant change in the backbone structure is apparent in the conformations of Loop-7 and Loop-8. In this variant, Loop-7, including the Loop-7 α-helix, is pulled toward the active site (FIG. 16B). A portion of Loop-8 is similarly pulled toward the active site. Loop-8 also participates in the dimer interface, but the cross-interface interactions are all retained in the L7ep-3a mutant.

The binding site for the substrate in wild-type PTE is divided into the large-group pocket (His-254, His-257, Leu-271, and Met-317), the leaving-group pocket (Trp-131, Phe-132, Phe-306, and Tyr-309), and the small-group pocket (Gly-60, Ile-106, Lue-303 and Ser-308).(50) The mutations H257Y and S308L, coupled with the shifting of the Loop-7 α-helix, have induced significant changes in the substrate binding pockets in the active site of the L7ep-3a mutant. The side-chain of Tyr-309 is repositioned so that the phenolic group now extends into the active site rather than towards Loop-7, as previously observed in the structure of wild-type PTE (FIGS. 16B and 17).

FIG. 17 depicts the substrate binding pockets of wild-type (white) and L7ep-3a (grey). The large-group pocket residues are His-254, His-257, Ile-271, and Met-317. The small-group pocket residues are Gly-60, Ile-106, Leu-303, and Ser-308. The leaving group pocket resides are Trp-131, Phe-132, Phe-306 and Tyr-309. The Wild-type structure (PDB id: 1DPM) is shown with the inhibitor, diethyl 4-methylbenzylphosphonate, bound in the active site.

The reorientation of Tyr-309, along with the substitution of a tyrosine for His-257 and the repositioning of Leu-271 into the active site, has dramatically compressed the size of the large-group and leaving-group pockets. The leaving-group pocket is also constricted by the presence of the S308L mutation, which adds bulk to both the leaving-group and small-group pockets. However, the apparent contraction of the leaving-group pocket is partially relieved by the F132V mutation. Similarly, the I106C mutation opens additional space to the small-group pocket.

Three-Dimensional Structure of L7ep-3a I106G. In an effort to understand the physical basis for the observed improvement in the catalytic activity of L7ep-3a I106G, the three-dimensional structure was solved by X-ray crystallography (PDB id: 4ZSU). The core structure is very similar to wild-type PTE (Cα RMSD=0.66 Å) and the loop structure matches that observed with L7ep-3a.

Example 33

Computational Docking of High Energy Intermediates. The pentavalent high-energy reaction intermediate states for the hydrolysis of VX and VR were computationally docked into the three-dimensional structures of wild-type PTE (PDB id: 1DPM), H254Q/H257F (PDB id: 2OQL), L7ep-3a (PDB id: 4ZST), and L7ep-3aG (PDB id: 4ZSU). The high energy intermediate states for the hydrolysis of the R_(P)- and S_(P)-enantiomers were manually generated as trigonal bipyrimidal structures with the attacking hydroxyl group protonated and the original phosphoryl oxygen substituent carrying a full negative charge using ChemBio Ultra 14.0. Computational docking was done using the program AutoDock Vina.(49) The appropriateness of the docked poses was evaluated by the value of the distance of the attacking hydroxyl group from the α- and β-metal ions, the distance of the phosphoryl oxygen from the β-metal and the orientation of the side ester substituents into the large and small group pockets contained in the active site of PTE.

Example 34

Evaluation of New V-agent Analogs. The majority of research targeting the catalytic hydrolysis of organophosphorus nerve agents must be done using analogs for both regulatory and safety reasons. Intrinsic to the use of substrate analogs is the imperfect representation of catalytic activity with the authentic nerve agent. To address which structural factors of the VR and VX analogs are most significant, the compounds DMVX, DEVR and OMVR were synthesized and analyzed as substrates for the optimized mutants of PTE and compared with the ability of these mutants to hydrolyze the most toxic forms of VR and VX. The catalytic activity using these compounds was determined with a series of variants for which the hydrolysis of authentic nerve agents was available (Table 15). Wild-type PTE has a much lower catalytic activity with DMVX (k_(cat)/K_(m)=1.9×101 M⁻¹ s⁻¹) than was observed with DEVX (k_(cat)/K_(m) 1.2×103 M⁻¹ s⁻¹). The best variant with DMVX was L7ep-3a, which has a k_(cat)=28 s⁻¹ and a k_(cat)/K_(m)=1.3×104 M⁻¹ s⁻¹. These values are 1,300- and 680-fold better, respectively, than wild-type PTE. Wild-type PTE exhibited better catalytic activity with DEVR (k_(cat)/K_(m)=5.6×102 M−¹ s⁻¹). L7ep-3a also had the best catalytic activity with this analog (k_(cat)/K_(m)=1.5×104 M⁻¹ s⁻¹). With the exception of wild-type PTE (k_(cat)/K_(m)=6.8×101 M⁻¹ s⁻¹), racemic OMVR gave the least activity for most of the variants tested. The combination of poor solubility of this compound and high K_(m) values limited analysis to the determination of k_(cat)/K_(m) for most variants. The best mutant for the hydrolysis of OMVR was L7ep-3a with a k_(cat)/K_(m)=5.8×102 M⁻¹ s⁻¹. However, given the switch in stereochemical preference, it is highly likely that L7ep-3a I106G has the best catalytic activity with the R_(P)-enantiomer of OMVR (which corresponds to the same relative stereochemistry as the S_(P)-enantiomer of VR.

TABLE 15 Kinetic constants for PTE variants with V-agent analogs¹. DMVX DEVR OMVR² k_(cat) K_(m) k_(cat)/K_(m) k_(cat) K_(m) k_(cat)/K_(m) k_(cat) K_(m) k_(cat)/K_(m) Enzyme (s⁻¹) (mM) (M⁻¹s⁻¹) (s⁻¹) (mM) (M⁻¹s⁻¹) (s⁻¹) (mM) (M⁻¹s⁻¹) Wild-type 0.021 1.1 1.9 × 10¹ 0.201 0.38 5.6 × 10² nd nd 6.8 × 10¹ QF 0.21 0.80 2.6 × 10² 0.82 0.37 2.2 × 10³ 0.15 1.7 7.1 × 10¹ CVQFL 17 3.7 4.4 × 10³ 1.49 0.19 7.8 × 10³ nd nd 2.1 × 10² VRN-VQFL 5.1 0.91 5.5 × 10³ 3.1 0.36 8.7 × 10³ nd nd 5.1 × 10² VRN-VQF-L308S* 3.0 1.8 1.6 × 10³ 1.94 0.21 9.2 × 10³ nd nd 1.4 × 10² VRN-VQFL-I106G 0.68 1.6 4.4 × 10² 0.47 0.8 5.9 × 10² nd nd 3.3 × 10² VRN-VQFL- 0.3 1.15 2.6 × 10² 0.115 0.97 1.2 × 10² nd nd 1.9 × 10² I106G/L308S L7ep-3a 28 2.1 1.3 × 10⁴ 6.8 0.44 1.5 × 10⁴ 1.0 1.5 5.8 × 10² L7ep-3a I106G nd nd 1.4 × 10³ 4 6 6.7 × 10² nd nd 2.7 × 10² *L308S mutation is a revertant to the wild-type amino acid sequence. ¹Errors from curve fitting were less than 10% except for k_(cat) and K_(m) for L7ep3aG with DEVR. ²k_(cat)/K_(m) was determined from linear fit at low concentration of racemic substrate.

Comparison of Substrate Analogs. The VX analog DEVX was successfully used to identify PTE variants for the hydrolysis of VX, but it over-estimated the activity of the wild-type enzyme and failed to detect a 100-fold increase in the catalytic activity with the QF variant.(37) DEVX was initially synthesized to mimic the O-ethyl substituent in VX, but the bulk of the diethyl phosphorus center is larger than the volume of the methylphosphonate moiety of VX. DMVX also contains an achiral phosphorus center, but the volume of the dimethyl center is more representative of authentic VX. The catalytic activity of the PTE variants with DMVX was surprisingly low, but this analog captures the much lower catalytic activity of wild-type PTE for the hydrolysis of VX and the substantial increase in activity with the QF variant. The catalytic properties for the hydrolysis of DMVX are also able to predict the high k_(cat) for the hydrolysis of VX by the L7ep-3a variant. While DEVX was intended to ensure accommodation of the larger O-ethyl substituent, the data for DMVX suggests that for mimicking VX, the overall size of the phosphorus center is more important. While the asymmetry of the phosphonate center is obviously a major contributor to the catalytic activity using VX as a substrate, the dimethyl center provided a reasonable prediction of the catalytic activity.

The compound DEVR was synthesized to test the significance of the diethylamino vs. diisopropylamino groups contained within the VR and VX leaving groups, respectively. The smaller leaving group of DEVR resulted in 2-fold less activity compared to DEVX for wild-type PTE. Similar differences were obtained for most of the other variants. L7ep-3a I106G was the only variant where the catalytic activity with DEVR was less than 10% of the catalytic activity with DEVX. The relative activity between variants was similar with either leaving group but the reduced activity, especially manifested in the value of k_(cat), suggests that the interactions of the enzyme with the leaving group maybe partially responsible for aligning the phosphorus center for nucleophilic attack. The smaller leaving group probably contributes to the lower enzymatic activity observed with VR, but comparison to the catalytic activity with DEVR also highlights the dominance of the phosphorus center. The introduction of I106G in the L7ep-3a variant resulted in a 23-fold loss of activity with DEVR, but the activity with authentic VR was improved.

In an attempt to better reflect the asymmetric phosphorus center of VR, the analog OMVR was synthesized. The PTE variants exhibited the least activity with the analog OMVR, which employs a slightly larger but asymmetric phosphorus center and the authentic leaving group of VR. Kinetic constants with racemic OMVR are about an order of magnitude smaller than is obtained with authentic VR, but the relative activity between variants is much more consistent than is seen with the other analogs. VRN-VQFL and L7ep-3a both have substantially better activity than wild-type PTE or QF for both OMVR and authentic VR. Introduction of I106G or removal of S308L in the VRN-VQFL variant resulted in somewhat diminished rates for both authentic VR and OMVR.

Example 35

Active Site Hydrogen Bonding Network. The kcat values for wild-type PTE with phosphorothiolate substrates are approximately 104-fold lower than that with its best substrates.(37, 51) In the hydrolysis of substrates such as paraoxon there is no need to protonate the leaving group.(52)

FIG. 18 depicts the metal center of wild-type PTE (A), QF (B), and L7ep-3a (C) variants. The residues binding to the α-metal (His-55, His-57, and Asp-301), the β-metal (His-201 and His-230), and the bridging carboxylated Lys-169 are shown. The proton shuttle residues His-257, His-254, and Asp-233 are also shown. The wild-type structure is obtained from PDB id: 1DPM and the QF structure is obtained from PDB id: 2OQL.

In the proposed reaction mechanism for wild-type PTE, the proton from the attacking nucleophilic water is passed to Asp-301, and, in turn, to His-254 (FIG. 18A).(53) The proton is then transferred to Asp-233 and on to bulk solvent. The variant QF has been postulated to have significantly improved catalytic activity with VX in part because of the disruption of this proton shuttle. In the crystal structure of the mutant QF, His-254 of the wild-type enzyme is a glutamine, which cannot participate in proton shuttling, and Asp-233 is moved out of hydrogen bonding distance (FIG. 18B). It is thought that the “trapping” of the proton in the active site is useful for the hydrolysis of slow substrates like VX, where protonation of the leaving group will contribute to improved k_(cat) values. The crystal structure of L7ep-3a, which has a kcat value for the hydrolysis of VX about an order of magnitude higher than QF, shows a remarkable rearrangement of the hydrogen bonding pattern in the active site. In L7ep-3a, Gln-254 hydrogen bonds to Asp-301, and Asp-233 has moved back into hydrogen bonding distance to Gln-254. Tyr-257 is also hydrogen bonded to Asp-301. The dramatic alteration of the hydrogen bonding network of Asp-301 results in the displacement of the nucleophile water toward the α-metal. This asymmetrical binding to the binuclear metal center is likely to result in the bridging hydroxyl being a stronger nucleophile. In the L7ep-3a I106G mutant, a similar hydrogen bonding pattern is observed, but Asp-233 is moved out of hydrogen bonding distance and the displacement of the bridging hydroxyl is not nearly as pronounced. The asymmetric positioning of the bridging hydroxyl has previously been observed in the crystal structure of dihydroorotase in the presence of bound dihydroorotate.(54)

Example 36

Docking of Substrates in the Active Site. In an effort to gain insight into the altered activity of L7ep-3a and L7ep-3a I106G, the substrates VX and VR were docked into the active site using the program AutoDock Vina. Computational docking was conducted using the trigonal bipyrimidal intermediates formed during the hydrolysis of both enantiomers of these compounds.(55) Productive poses were assessed by the placement of the attacking hydroxyl group between the two metal ions and the orientation of the phosphoryl oxygen toward the β-metal.(56) For the wild-type and QF variants both enantiomers of VX and VR could be reasonably docked into the active site (data not shown). However, for L7ep-3a and L7ep-3a I106G, only the S_(P)-enantiomer of VR could be reasonable positioned in the active site. For both of these variants, the constriction of the active site and the repositioning of Tyr-309 appear to play important roles in the activity against the V-agents (FIG. 19).

FIG. 19 depicts (A) S_(P)-VX docked in thee active site of L7ep-3a. (B) S_(P)-VR docked into the active site of L7ep-3a I106G. The substrate binding residues are shown. The distances from Tyr-309 and Asp-301 are shown in units of Ångstoms.

The mutation F132V provides the extra room to accommodate the isopropyl amino group of VX. This effect is not as obvious with the smaller substituent contained within the leaving group in VR. The changes in the active site also enable the sulfur and the nitrogen of the leaving group to potentially hydrogen bond with the side chain phenol of Tyr-309, suggesting that this interaction may be partially responsible for the dramatically improved activity. The additional space in the small-group pocket due to the I106G mutation accommodates the isobutyl group in S_(P)-VR, while the combination of the H257Y mutation and repositioning of Tyr-309 make binding of the R_(P)-enantiomer more difficult.

The determination of the three-dimensional structure of the L7ep-3a mutant has led to a greater understanding of the underlying mechanisms by which the hydrolysis of V-agents is enhanced.

FIG. 20 depicts an equation showing the interaction between S_(P)-VR and L7ep3a-PTE resulting in hydrolysis of S_(P)-VR.

The determination of this structure has directly led to the rational construction of the new L7ep-3a I106G mutant, which is enhanced 620-fold for the hydrolysis of the toxic S_(P)-enantiomer of VR, relative to the wild-type enzyme. Previous work with the insecticide demeton-S demonstrated the importance of the leaving group on the catalytic activity of PTE, and our results with the new analogs of VR and VX has further demonstrated that even small changes in the leaving group can have dramatic effect on the activity of the enzyme.(37) The crystal structures of L7ep-3a and L7ep-3a I106G have provided a physical basis for these observations. The computational docking results have suggested how the remodeled active site is able to exploit hydrogen bonding interactions with Tyr-309. The disruption of the proton shuttle, along with new hydrogen bonds to Asp-301, are apparently able to enhance the attack of the bridging hydroxide on phosphorothiolate substrates. The initial data with the new racemic analog OMVR suggests that the combined asymmetric phosphorus center and the authentic leaving group of VR will allow for much more accurate predictions of the activity against VR and enable the more rapid development of new variants that are more fully optimized for the hydrolysis of VR.

All of the compositions and methods disclosed and claimed herein can be made and executed without undue experimentation in light of the present disclosure. While the compositions and methods of this disclosure have been described in terms of preferred embodiments, it will be apparent to those of skill in the art that variations can be applied to the compositions and methods and in the steps or in the sequence of steps of the methods described herein without departing from the concept, spirit and scope of the disclosure. More specifically, it will be apparent that certain agents which are both chemically and physiologically related can be substituted for the agents described herein while the same or similar results would be achieved. All such similar substitutes and modifications apparent to those skilled in the art are deemed to be within the spirit, scope and concept of the disclosure as defined by the appended claims.

REFERENCES

-   1. Maxwell, D. M.; Brecht, K. M.; Koplovitz, I.; Sweeney, R. E. Mol.     Toxicol. 2006, 80, 756. -   2. Leikin, J. B.; Thomas, R. G.; Walter, F. G.; Klein, R.;     Meislin, H. W. Crit. Care. Med. 2002, 30, 2346. -   3. Columbus, I.; Waysbort, D.; Marcovitch, I.; Yehezkel, L.;     Mizrahi, D. M. Environ. Sci. Technol. 2012, 46, 3921. -   4. Yang, Y. C. Chem. Ind. 1995, 9, 334. -   5. Yang, Y. C. Accounts Chem. Res. 1999, 32, 109. -   6. Saxina, A.; Sun, W.; Fedorko, J. M.; Koplovitz, I.; Doctor, B. P.     Biochem. Pharmacol. 2011, 81, 164. -   7. Ashani, Y.; Pistinner, S. Toxicol. Sci. 2004, 77, 358. -   8. Saxena, A.; Tipparaju, P.; Luo, C.; Doctor, B. P. Process     Biochem. 2010, 45, 1313. -   9. Cheng, T.-C.; Liu, L.; Wang, B.; Wu, J.; DeFrank, J. J.;     Anderson, D. M.; Rastogi, V. K.; Hamilton, A. B. J. Ind. Microbiol.     Biotechnol. 1997, 18, 49. -   10. Melzer, M.; Chen, J. C.-H.; Heidenreich, A; Gab, J; Koller, M;     Kehe, K; Blum, M.-M. J. Am. Chem. Soc. 2009, 131, 17226 -   11. Kirby, S. D.; Norris, J. R.; Smith, J. R.; Bahnson, B. J.;     Cerasoli, D. M. Chem. Biol. Interact. 2012, 203, 181. -   12. Gupta, R. D.; Goldsmith, M.; Ashani, Y.; Simo, Y.; Mullokandov,     G.; Bar, H.; Ben-David, M.; Leader, H.; Margalit, R.; Silman, I.;     Sussman, J. L.; Tawfik, D. S. Nat. Chem. Biol. 2011, 7, 120 -   13. Tsai, P.-C.; Fox, N.; Bigley, A. N.; Harvey, S. P.;     Barondeau, D. P.; Raushel, F. M. Biochemistry 2012, 51, 6463. -   14. Lai, K.; Grimsley, J. K.; Kuhlmann, B. D.; Scapozza, L.;     Harvey, S. P.; DeFrank, J. J.; Kolakowski, J. E.; Wild, J. R. Chimia     1996, 50, 430. -   15. Caldwell, S. R.; Newcomb, J. R.; Schlecht, K. A.; Raushel, F. M.     Biochemistry 1991, 30, 7438. -   16. Benschop, H. P.; De Jong, L. P. A. Accounts Chem. Res. 1988, 21,     368. -   17. Ordentlich, A.; Barak, D.; Sod-Moriah, G.; Kaplan, D.; Mizrahi,     D.; Segall, Y.; Kronman, C.; Karton, Y.; Lazar, A.; Marcus, D.;     Velan, B.; Shafferman, A. Biochemistry 2004, 43, 11255. -   18. Tsai, P. C.; Bigley, A, N.; Li, Y.; Ghanem, E.; Cadieux, C. L.;     Kasten, S. A.; Reeves, T. E.; Cerasoli, D. M.; Raushel, F. M.     Biochemistry 2010, 49, 7978. -   19. Rastogi, V. K.; DeFrank, J. J.; Cheng, T.; Wild, J. R. Biochem.     Bioph. Res. Co. 1997, 241, 294. -   20. Hong, S.-B.; Raushel, F. M. Biochemistry 1996, 35, 10904. -   21. Vanhooke, J. L.; Benning, M. M.; Raushel, F. M.; Holden, H. M.     Biochemistry 1996, 35, 6020. -   22. Chen-Goodspeed, M.; Sogorb, M. A.; Wu, F.; Hong, S.-B.;     Raushel, F. M. Biochemistry 2001, 40, 1325. -   23. Afriat-Jurnou, L; Jackson, C. J.; Tawfik, D. S. Biochemistry,     2012, 51, 6047. -   24. Reeves, T. E.; Wales, M. E.; Grimsley, J. K.; Li, P.;     Cerasoli, D. M.; Wild, J. R. Protein Eng. Des. Sel. 2008, 21, 405. -   25. Schofield, D. A.; DiNovo, A. A. J. Appl. Microbiol. 2010, 109,     548 -   26. Horton, R. M.; Hunt, H. D.; Ho, S. N.; Pullen, J. K.;     Pease, L. R. Gene 1989 77, 61 -   27. Goldsmith, M.; Kiss, C.; Bradbury, A. R. M.; Tawfik, D. S.     Protein Eng. Del. Sel. 2007, 20, 315. -   28. Cho, C. M.; Mulchandani, A.; Chen, W. Protein Eng. Del. Sel.     2006, 19, 99. -   29. Roodveldt, C.; Tawfik, D. S. Protein Eng. Des. Sel. 2005, 18,     51. -   30. Aubert, S. D.; Li, Y.; Raushel, F. M. Biochemistry 2004, 43,     5707. -   31. Shaka, A. J.; Keeler, J.; Freeman, J. R. J. Magn. Reson. 1983,     53, 313. -   32. Batley, M.; Redmond, J. W. J. Magn. Reson. 1982, 49, 172. -   33. Benschop, H. P., and De Jong, L. P. A. (1988) Nerve agent     stereoisomers: analysis, isolation and toxicology, Acc. Chem. Res.     21, 368-374. -   34. Rosman, Y., Eisenkraft, A., Milk, N., Shiyovich, A., Ophir, N.,     Shrot, S., Kreiss, Y., and Kassirer, M. (2014) Lessons learned from     the Syrian sarin attack: Evaluation of a clinical syndrome through     social media, Ann. Intern. Med. 160, 644-648. -   35. Leikin, J. B., Thomas, R. G., Walter, F. G., Klein, R., and     Meislin, H. W. (2002) A review of nerve agent exposure for the     critical care physician, Crit. Care Med. 30, 2346-2354. -   36. Columbus, I., Waysbort, D., Marcovitch, I., Yehezkel, L., and     Mizrahi, D. M. (2012) VX fate on common matrices: evaporation versus     degradation, Environ. Sci. Technol. 46, 3921-3927. -   37. Bigley, A. N., Xu, C., Henderson, T. J., Harvey, S. P., and     Raushel, F. M. (2013) Enzymatic neutralization of the chemical     warfare agent VX: evolution of phosphotriesterase for     phosphorothiolate hydrolysis, J. Am. Chem. Soc. 135, 10426-10432. -   38. Tsai, P. C., Fox, N., Bigley, A. N., Harvey, S. P.,     Barondeau, D. P., and Raushel, F. M. (2012) Enzymes for the homeland     defense: Optimizing phosphotriesterase for the hydrolysis of     organophosphate nerve agents, Biochemistry 51, 6463-6475. -   39. Tsai, P. C., Bigley, A., Li, Y., Ghanem, E., Cadieux, C. L.,     Kasten, S. A., Reeves, T. E., Cerasoli, D. M., and     Raushel, F. M. (2010) Stereoselective hydrolysis of organophosphate     nerve agents by the bacterial phosphotriesterase, Biochemistry 49,     7978-7987. -   40. Mee-Hie Cho, C., Mulchandani, A., and Chen, W. (2006) Functional     analysis of organophosphorus hydrolase variants with high     degradation activity towards organophosphate pesticides, Protein     Eng., Des. Sel. 19, 99-105. -   41. Roodveldt, C., and Tawfik, D. S. (2005) Directed evolution of     phosphotriesterase from Pseudomonas diminuta for heterologous     expression in Escherichia coli results in stabilization of the     metal-free state, Protein Eng., Des. Sel. 18, 51-58. -   42. Rastogi, V. K., DeFrank, J. J., Cheng, T. C., and     Wild, J. R. (1997) Enzymatic hydrolysis of Russian-VX by     organophosphorus hydrolase, Biochem. Biophys. Res. Commun. 241,     294-296. -   43. Cherny, I., Greisen, P., Jr., Ashani, Y., Khare, S. D.,     Oberdorfer, G., Leader, H., Baker, D., and Tawfik, D. S. (2013)     Engineering V-type nerve agents detoxifying enzymes using     computationally focused libraries, ACS chem. Biol. 8, 2394-2403. -   44. Amitai, G., Ashani, Y., Grunfeld, Y., Kalir, A., and     Cohen, S. (1976) Synthesis and properties of     2-S—(N,N-dialkylamino)ethyl)thio-1,3,2-dioxaphosphorinane 2-oxide     and of the corresponding quaternary derivatives as potential     nontoxic antiglaucoma agents, J. Med. Chem. 19, 810-813. -   45. Michaelis, L., and Menten, M. L. (1913) Die kinetik der     invertinwirkung, Biochem. Z. 49, 333-369. -   46. Otwinowski Z, M. W. (1997) Processing of X-ray diffraction data     collected in oscillation mode, Methods Enzymol. 276A, 307-326. -   47. Adams, P. D., Afonine, P. V., Bunkoczi, G., Chen, V. B.,     Davis, I. W., Echols, N., Headd, J. J., Hung, L.-W., Kapral, G. J.,     Grosse-Kunstleve, R. W., McCoy, A. J., Moriarty, N. W., Oeffner, R.,     Read, R. J., Richardson, D. C., Richardson, J. S., Terwilliger, T.     C., and Zwart, P. H. (2010) PHENIX: a comprehensive Python-based     system for macromolecular structure solution, Acta Crystallogr.,     Sect. D: Biol. Crystallogr. 66, 213-221. -   48. Emsley, P., and Cowtan, K. (2004) Coot: model-building tools for     molecular graphics, Acta Crystallogr., Sect. D: Biol. Crystallogr.     60, 2126-2132. -   49. Trott, O., and Olson, A. J. (2010) AutoDock Vina: Improving the     speed and accuracy of docking with a new scoring function, efficient     optimization, and multithreading, J. Comput. Chem. 31, 455-461. -   50. Chen-Goodspeed, M., Sogorb, M. A., Wu, F., Hong, S. B., and     Raushel, F. M. (2001) Structural determinants of the substrate and     stereochemical specificity of phosphotriesterase, Biochemistry 40,     1325-1331. -   51. Caldwell, S. R., Newcomb, J. R., Schlecht, K. A., and     Raushel, F. M. (1991) Limits of diffusion in the hydrolysis of     substrates by the phosphotriesterase from Pseudomonas diminuta,     Biochemistry 30, 7438-7444. -   52. Hong, S. B., and Raushel, F. M. (1996) Metal-substrate     interactions facilitate the catalytic activity of the bacterial     phosphotriesterase, Biochemistry 35, 10904-10912. -   53. Aubert, S. D., Li, Y., and Raushel, F. M. (2004) Mechanism for     the hydrolysis of organophosphates by the bacterial     phosphotriesterase, Biochemistry 43, 5707-5715. -   54. Thoden, J. B., Phillips, G. N., Neal, T. M., Raushel, F. M., and     Holden, H. M. (2001) Molecular Structure of Dihydroorotase: A     paradigm for catalysis through the use of a binuclear metal center,     Biochemistry 40, 6989-6997. -   55. Caldwell, S. R., Raushel, F. M., Weiss, P. M., and     Cleland, W. W. (1991) Transition-state structures for enzymatic and     alkaline phosphotriester hydrolysis, Biochemistry 30, 7444-7450. -   56. Vanhooke, J. L., Benning, M. M., Raushel, F. M., and     Holden, H. M. (1996) Three-dimensional structure of the     zinc-containing phosphotriesterase with the bound substrate analog     diethyl 4-methylbenzylphosphonate, Biochemistry 35, 6020-6025. 

What is claimed is:
 1. The synthetic amino acid sequence comprising the synthetic amino acid sequence of L7ep-3a (SEQ ID NO.: 5).
 2. A synthetic DNA sequence encoding the synthetic amino acid sequence of claim
 1. 3. A synthetic cDNA sequence comprising the coding sequence of the synthetic DNA sequence of claim
 2. 4. A plasmid comprising the synthetic DNA sequence of claim
 2. 5. A method of hydrolysis of a organophosphate nerve agent comprising contacting an organophosphate nerve agent with the synthetic amino acid sequence of claim 1 (SEQ ID NO.:5); and hydrolyzing the organophosphate nerve agent.
 6. The method of hydrolysis of claim 5, wherein the organophosphate is VX.
 7. The method of hydrolysis of claim 5, wherein the organophosphate is VR.
 8. The method of hydrolysis of claim 5, wherein the organophosphate is selected from the group consisting of GB, GD, and GF.
 9. A system for detoxifying an organophosphate nerve agent comprising contacting the synthetic amino acid sequence of claim 1 with an organophosphate nerve agent.
 10. A kit for detoxifying an organophosphate nerve agent comprising the synthetic amino acid sequence of claim
 1. 11. A synthetic amino acid sequence comprising the synthetic amino acid sequence of L7ep-3a I106G (SEQ ID NO.: 6).
 12. A synthetic DNA sequence encoding the synthetic amino acid sequence of claim
 11. 13. A synthetic cDNA sequence comprising the coding sequence of the synthetic DNA sequence of claim
 12. 14. A plasmid comprising the synthetic DNA sequence of claim
 12. 15. A method of hydrolysis of an organophosphate nerve agent comprising contacting an organophosphate nerve agent with the synthetic amino acid sequence of claim 11 (SEQ ID NO.: 6); and hydrolyzing the organophosphate nerve agent.
 16. The method of hydrolysis of claim 15, wherein the organophosphate is VX.
 17. The method of hydrolysis of claim 15, wherein the organophosphate is VR.
 18. The method of hydrolysis of claim 15, wherein the organophosphate is selected from the group consisting of GB, GD, and GF.
 19. A system for detoxifying an organophosphate nerve agent comprising contacting the synthetic amino acid sequence of claim 11 with an organophosphate nerve agent.
 20. A kit for detoxifying an organophosphate nerve agent comprising the synthetic amino acid sequence of claim
 11. 21. A method of producing variants of phosphotriesterase, wherein the variants are capable of detoxifying an organophosphate nerve agent, comprising the steps of: obtaining a PTE gene; inserting the PTE gene into a vector; preparing a series of sequential mutational libraries wherein the PTE gene encodes a synthetic amino acid sequence of L7ep-3a I106G (SEQ ID NO.: 6); expressing the variant as a protein; screening the variant for catalytic activity against one selected from the group consisting of DEVX, DMVX, DEVR, and OMVR to determine the hydrolytic activity; and selecting the variant for use in hydrolysis of an organophosphate nerve agent based upon its hydrolytic activity.
 22. The method of claim 21 wherein the variant synthetic amino acid sequence is at least 80% homogenous to the synthetic amino acid sequence of SEQ ID NO.:
 6. 23. A method of producing variants of phosphotriesterase, wherein the variants are capable of detoxifying an organophosphate nerve agent, comprising the steps of: obtaining a PTE gene; inserting the PTE gene into a vector; preparing a series of sequential mutational libraries wherein the PTE gene encodes a synthetic amino acid sequence comprising the mutations I106C, F132V, H254Q, H257Y, A270V, L272M, I274N, and S308L (SEQ ID NO.: 5); expressing the variant as a protein; screening the variant for catalytic activity against one selected from the group consisting of DEVX, DMVX, DEVR, and OMVR to determine the hydrolytic activity; and selecting the variant for use in hydrolysis of an organophosphate nerve agent based upon its hydrolytic activity.
 24. The method of claim 23 wherein the variant comprising the mutations I106C, F132V, H254Q, H257Y, A270V, L272M, I274N, and S308L synthetic amino acid sequence is at least 80% homogenous to the synthetic amino acid sequence of SEQ ID NO.:
 5. 